Biosynthetic proline/alanine random coil polypeptides and their uses

ABSTRACT

The present invention relates to a biosynthetic random coil polypeptide or a biosynthetic random coil polypeptide segment or biosynthetic conjugate, in which the biosynthetic random coil polypeptide, the biosynthetic random coil polypeptide segment, or the biosynthetic conjugate comprises an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein the amino acid sequence consists of at least about 50 proline (Pro) and alanine (Ala) amino acid residues. The at least about 50 proline (Pro) and alanine (Ala) amino acid residues may be (a) fconstituent(s) of a heterologous polypeptide or an heterologous polypeptide construct. Also uses and methods of use of these biosynthetic random coil polypeptides or polypeptide segments or conjugates are described.

CROSS-REFERENCE TO RELATED PATENT APPLICATIONS

This application is a Divisional of U.S. patent application Ser. No. 14/939,626, filed Nov. 12, 2015, which is a Divisional of U.S. application Ser. No. 13/697,569, filed Nov. 13, 2012, now U.S. Pat. No. 9,221,882, which is the U.S. National Phase of International Patent Application No. PCT/EP2011/058307, filed May 20, 2011, which claims priority from U.S. Provisional Patent Application No. 61/428,016, filed Dec. 29, 2010, and European Patent Application No. 10163564.7, filed May 21, 2010. The foregoing applications are incorporated herein by reference in their entirety.

This application contains a Sequence Listing which has been submitted in ASCII format via EFS-Web and is hereby incorporated by reference in its entirety.

The present invention relates to a biosynthetic random coil polypeptide or a biosynthetic random coil polypeptide segment or a conjugate, said biosynthetic random coil polypeptide or a biosynthetic random coil polypeptide segment or a conjugate comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least about 50 proline (Pro) and alanine (Ala) amino acid residues. Said at least about 50 proline (Pro) and alanine (Ala) amino acid residues may be (a) constituent(s) of a heterologous polypeptide or an heterologous polypeptide construct. Also uses and methods of use of these biosynthetic random coil polypeptides, said polypeptide segments or said conjugates are described. The uses may, inter alia, comprise medical uses, diagnostic uses or uses in the food industry as well as other industrial applications, like in the paper industry, in oil recovery and the like. The present invention relates, also, to (a) specific use(s) of the herein provided biosynthetic random coil polypeptide or biosynthetic random coil polypeptide segment or conjugates, said biosynthetic random coil polypeptide or biosynthetic random coil polypeptide segment or conjugates comprising an amino acid sequence consisting solely of proline and alanine amino acid residues. The amino acid sequence of the herein provided biosynthetic random coil polypeptide or biosynthetic random coil polypeptide segment consists of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350 or of at least about 400 proline (Pro) and alanine (Ala) amino acid residues. Said at least about 50, at least about 100, at least about 150, at least about 200, at least about 250, at least about 300, at least about 350 or at least about 400 proline (Pro) and alanine (Ala) amino acid residues are preferably (a) a constituent of a heterologous polypeptide or a heterologous polypeptide construct or are preferably (b) a constituent of a conjugate, like a drug conjugate, like a conjugate with a food or cosmetic ingredient or additive, like a conjugate with a biologically active compound or like a conjugate with a spectroscopically active compound. In particular, heterologous proteins are provided herein whereby these proteins comprise at least two domains, wherein a first domain of said at least two domains comprises an amino acid sequence having and/or mediating an activity, like a biological activity, and a second domain of said at least two domains comprising the biosynthetic random coil proline/alanine polypeptide or proline/alanine polypeptide segment of the present invention. The present invention relates in particular to a drug conjugate comprising (i) a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, and (ii) a drug selected from the group consisting of (a) a biologically active protein or a polypeptide that comprises or that is an amino acid sequence that has or mediates a biological activity and (b) a small molecule drug. A further subject of the present invention is a drug conjugate comprising the biosynthetic random coil proline/alanine polypeptide or proline/alanine polypeptide segment as provided herein and, additionally, (a) pharmaceutically or medically useful molecule(s), like small molecules, peptides or biomacromolecules (such as proteins, nucleic acids, carbohydrates, lipid vesicles) and the like, linked and/or coupled to said biosynthetic random coil proline/alanine polypeptide or proline/alanine polypeptide segment. Furthermore, nucleic acid molecules encoding the biosynthetic random coil polypeptide or polypeptide segment and/or the biologically active, heterologous proteins as well as vectors and cells comprising said nucleic acid molecules are disclosed. Furthermore, methods for the production of the herein described inventive biosynthetic random coil polypeptides or polypeptide segments and corresponding drug or food conjugates, i.e. conjugates comprising the herein defined biosynthetic random coil polypeptides or polypeptide segments and a food ingredient or a food additive, are disclosed. Also disclosed are corresponding conjugates (comprising as one constituent the herein disclosed biosynthetic random coil polypeptide or polypeptide segment) which comprise, inter alia, a cosmetic ingredient or additive or a biologically or spectroscopically active compound. In addition, the present invention provides compositions comprising the compounds of the invention (i.e. the herein disclosed the random coil polypeptides or random coil polypeptide segments comprising an amino acid sequence consisting solely of proline and alanine amino acid residues and nucleic acid molecules encoding the same) as well as specific uses of said random coil polypeptide or polypeptide segment, of the biologically active proteins comprising said random coil polype random coil polypeptides or random coil polypeptide segments ptides or random coil polypeptide segments, the drug conjugates, the food conjugates or the nucleic acid molecules, vectors and cells of the invention. Also methods of producing and/or obtaining the inventive biosynthetic random coil polypeptides or polypeptide segments as well as of producing and/or obtaining the inventive biologically active, heterologous proteins, and/or polypeptide constructs or drug conjugates are provided. In addition, medical, pharmaceutical as well as diagnostic uses are provided herein for the biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues (or for molecules and conjugates comprising the same) as defined herein. Such a medical or pharmaceutical use can comprise the use of said biosynthetic random coil polypeptide or polypeptide segment as plasma expander and the like. However, the means and methods provided herein are not limited to pharmaceutical, medical and biological uses but can also be employed in other industrial areas, like in the paper industry, in oil recovery, etc.

Rapid clearance from blood circulation by renal filtration is a typical property of small molecules (including small proteins and peptides). However, by expanding the apparent molecular dimensions beyond the pore size of the kidney glomeruli plasma half-life of therapeutic proteins can be extended to a medically useful range of several days. One strategy to achieve such an effect is chemical conjugation of the biologic with the synthetic polymer poly-ethylene glycol (PEG). This has led to several approved drugs, for example PEG-interferon alpha2a (Pegasys®), PEG-G-CSF (Neulasta®) and, recently, a PEGylated alphaTNF-Fab fragment (Cimzia®). Nevertheless, the “PEGylation” technology has several drawbacks: clinical grade PEG derivatives are expensive and their covalent coupling to a recombinant protein requires additional downstream processing and purification steps, thus lowering yield and raising the costs. Furthermore, PEG is not biodegradable, which can cause side effects such as vacuolation of kidney epithelium upon continuous treatment; see, e.g., Gaberc-Porekar (2008) Curr Opin Drug Discov Devel 11:242-50; Knop (2010) Angew Chem Int Ed Engl 49:6288-308 or Armstrong in: Veronese (Ed.), “PEGylated Protein Drugs: Basic Science and Clinical Applications”; Birkhauser Verlag, Basel 2009.

In order to overcome some of the drawbacks of PEG technology, certain recombinant polypeptide mimetics have been provided in the art, some of which are based on naturally occurring amino acid sequences or synthetic amino acid stretches.

Most natural amino acid sequences do not behave like an ideal random chain in physiological solution because they either tend to adopt a folded conformation (secondary structure) or, if unfolded, they usually are insoluble and form aggregates. In fact, most of the classical experiments to investigate the random chain behaviour of polypeptides were conducted under denaturing conditions, i.e. in the presence of chemical denaturants like urea or guanidinium chloride (see, e.g., Cantor (1980) Biophysical Chemistry. W.H. Freeman and Company, New York). Hence, such technologies generally rest upon peculiar amino acid sequences that resist folding, aggregation as well as unspecific adsorption and, thus, provide stable random chains under physiological buffer conditions and temperature even if genetically fused to a folded therapeutic protein domain. Under these circumstances, such recombinant PEG mimetics can confer a size increase much larger than one would normally expect on the basis of their molecular mass alone, eventually retarding kidney filtration and effectively extending plasma half-life of the attached biologic by considerable factors.

A lot of these technologies have, however, further caveats and disadvantages.

For example, naturally occurring repetitive amino acid sequences have been tested for their usefulness in medical sciences and in pharmaceutical approaches. One of these approaches relates to the trans-sialidase of Trypanosoma cruzi. It contains a 680 amino acid residue catalytic domain followed by a C-terminal repetitive domain, dubbed “shed acute phase antigen” (SAPA), which comprises a variable number of 12mer amino acid repeats. Pharmacokinetic (PK) studies in mice of the trans-sialidase containing 13 hydrophilic and (at physiological pH) negatively charged corresponding amino acid repeats having the natural sequence DSSAHSTPSTPA revealed a five-fold longer plasma half-life compared to the recombinant enzyme from which the C-terminal repetitive sequence had been deleted (Buscaglia (1999) Blood 93:2025-32). A similar half-life extending effect was observed after fusion of the same trans-sialidase, i.e. its 76 kDa catalytic domain, with 13 charged amino acid repeats of the sequence EPKSA that were found in the Trypanosoma cruzi protein antigen 13. Both the repeats from SAPA and from the antigen 13 were able to prolong the plasma half-life of the heterologous protein gluthatione S-transferase (GST) from Schistosoma japonicum by a factor 7-8 after genetic fusion to both C-termini of this homo-dimeric enzyme (see Buscaglia, loc.cit.). Yet, while these naturally occurring repetitive amino acid sequences from human pathogens in principle may appear attractive to optimize the pharmacokinetics of therapeutic proteins they were found to be highly immunogenic (see Affranchino (1989), Mol Biochem Parasitol 34:221-8 or Buscaglia (1998), J Infect Dis 1998; 177:431-6).

Another approach relates to the use of gelatin. Gelatin, hydrolyzed and denatured animal collagen, contains long stretches of Gly-Xaa-Yaa repeats, wherein Xaa and Yaa mostly constitute proline and 4-hydroxyproline, respectively. Succinylation of gelatin, primarily via the ε-amino groups of naturally interspersed lysine side chains, increases the hydrophilicity of this biopolymer and lowers its isoelectric point (pI). The intramolecular electrostatic repulsion between the negatively charged carboxylate groups of the modified side chains supposedly spreads out the molecule into a more or less extended conformation. The resulting expanded volume makes succinylated gelatin a macromolecule for use as plasma expander in humans and is, inter alia, marketed as Volplex® (Beacon Pharmaceuticals Ltd) or Gelofusine® (B. Braun Melsungen AG). Furthermore, a half-life extending effect was achieved by genetic fusion of granulocyte-colony-stimulating factor (G-CSF) to an artificial gelatin-like polypeptide (Huang (2010) Eur J Pharm Biopharm 74:435-41). To this end, all hydrophobic side chains in a natural gelatin were exchanged by hydrophilic residues, resulting in a 116 amino acid gelatin-like protein (GLK) comprising the amino acids G, P, E, Q, N, S, and K in varying order. G-CSF was fused at its N-terminus with 4 copies of this GLK sequence and secreted in Pichia pastoris. Pichia pastoris appeared as a favourable production organism for GLK fusion proteins; yet, if GLKs can also be produced in other organisms remains to be determined as it is known that recombinant gelatin fragments can be expressed with only low yield in E. coli, for example, as illustrated in Olsen (2003), Adv Drug Deliv Rev 55:1547-67.

Elastin is a component of the extracellular matrix in many tissues. It is formed from the soluble precursor tropoelastin, which consists of a hydrophilic Lys/Ala-rich domain and a hydrophobic, elastomeric domain with repetitive sequence. Enzymatic crosslinking of lysine side chains within the hydrophilic domain leads to insoluble elastin formation. Elastin-like polypeptides (ELPs) are artificially designed, repetitive amino acid sequences derived from the hydrophobic domain of tropoelastin. The most common repeat sequence motif of ELPs is V-P-G-X-G, wherein “X” can be any amino acid except Pro (MacEwan (2010) Biopolymers 94:60-77; Kim (2010) Adv Drug Deliv Rev 62:1468-78). Suitable ELPs can be fused with therapeutic proteins and produced in E. coli. Consequently, the ability of ELPs to form gel-like depots after injection can significantly prolong the in vivo half-life of an attached biologic, albeit by a mechanism different from the other unstructured polypeptides. Yet, ELP attachment can hamper the bioactivity of the fusion partner as demonstrated for the interleukin-1 receptor antagonist in an IL-1-induced lymphocyte proliferation bioassay (Shamji (2007) Arthritis Rheum. 11:3650-3661). In addition, ELPs are subject to degradation by endogenous proteases such as collagenase. Also, aggregated proteins are generally more susceptible to immunogenicity.

Further approaches relate to the use of polyanionic polymers. For example, polyglutamate (PG) has been chemically coupled to poorly soluble cytotoxic small molecule drugs for cancer treatment. A corresponding product would be Opaxio™, a paclitaxel drug conjugate currently in clinical phase III studies. Half-life of a paclitaxel PG conjugate was prolonged by a factor 3 to 14 in comparison with the unmodified compound (Singer (2005) J Control Release 109:120-6). Further fusion proteins, for example G-CSF fused at its N-terminus with a stretch of 175 consecutive Glu residues or IFN-alpha2 carrying at its C-terminus a PG tail of 84 residues, were produced in a soluble state in the cytoplasm of E. coli (see WO2002/077036). For efficient translation, the N-terminal fusion required a leader peptide, which was later removed by Tobacco Etch Virus (TEV) protease cleavage. Polyglutamate fusions of G-CSF and INFα2 showed bioactivity in cell culture assays. However, to date no pharmacokinetic data of these PG fusions have been reported. Also, the highly negative charge of PG fusions is a general disadvantage with respect to biomolecular interactions (e.g. binding of the target receptor or soluble factor) due to artificial electrostatic attraction or repulsion effects.

WO 2006/081249 describes a polypeptide sequence with about 2 to 500 repeat units of 3 to 6 amino acids, wherein G, N or Q represent the major constituents while minor constituents can be A, S, T, D or E. This amino acid composition allows integration of the glycosylation sequon Asn-Xaa-Ser/Thr (where Xaa is any amino acid except Pro) for N-linked glycosylation of the Asn side chain in eukaryotic expression systems. The increased macromolecular size of a resulting fusion protein, including posttranslational modification with bulky solvated carbohydrate structures, can extend the pharmacokinetics of the genetically conjugated protein. Such oligosaccharide attachments (“glycoengineering”) in general can both reduce susceptibility to proteolysis and increase the hydrodynamic volume (Sinclair (2005) J Pharm Sci 94:1626-35). A disadvantage is the intrinsic molecular heterogeneity of the glycosylated biomacromolecule, which causes additional effort during biotechnological production and quality control.

WO 2010/091122 (and WO 2007/103515) and Schellenberger (2009) Nat Biotechnol 27:1186-90 disclose unstructured non-repetitive amino acid polymers encompassing and comprising the residues P, E, S, T, A and G. This set of amino acids, which shows a composition not unlike the PSTAD repeat described further above, was systematically screened for sequences to yield a solvated polypeptide with large molecular size, suitable for biopharmaceutical development, by avoiding hydrophobic side chains—in particular F, I, L, M, V and W—that can give rise to aggregation and may cause an HLA/MHC-II mediated immune response. Also, potentially crosslinking Cys residues, the cationic amino acids K, R and H, which could interact with negatively charged cell membranes, and the amide side chains of N and Q, which are potentially prone to hydrolysis, were excluded (see Schellenberger (2009) loc. cit.). Synthetic gene libraries encoding non-repetitive sequences comprising the PESTAG set of residues, which were fused to the green fluorescent protein (GFP), were screened with respect to soluble expression levels in E. coli, and a resulting subset was further investigated for genetic stability, protein solubility, thermostability, aggregation tendency, and contaminant profile. Eventually, an 864 amino acid sequence containing 216 Ser residues (25.0 mole %), 72 Ala residues (8.3 mole %) and 144 amino acids (16.7 mole %) of each Pro, Thr, Glu, and Gly was further tested for fusion to the GLP-1 receptor agonist Exendin-4 (E-XTEN) and a few other biologics. The fusion proteins—typically carrying a cellulose binding domain, which was later cleaved off—were produced in a soluble state in the cytoplasm of E. coli and isolated. Investigation of of E-XTEN by circular dichroism (CD) spectroscopy revealed lack of secondary structure while during size exclusion chromatography (SEC) the fusion protein showed substantially less retention than expected for a 84 kDa protein, thus demonstrating an increased hydrodynamic volume (Schellenberg (2009) loc. cit.). The disordered structure of the PESTAG polypeptide and the associated increase in hydrodynamic radius may be favoured by the electrostatic repulsion between amino acids that carry a high net negative charge which are distributed across the XTEN sequence (see WO 2010/091122). However, a further study Geething (2010) PLoS One 2010; 5:e10175 demonstrated that XTEN decreases potency of its therapeutic fusion partner. In a cell culture assay, a glucagon XTEN fusion showed merely 15% bioactivity of the non-modified peptide. An even stronger loss in receptor affinity (17-fold increased EC₅₀) was described for an XTEN fusion of human growth hormone (hGH); see WO 2010/144502

Also glycine, as the smallest and structurally simplest amino acid, has been considered as the conformationally most flexible amino acid based on theoretical grounds; see, e.g. Schulz G E, Schirmer R H. Principles of Protein Structure. Springer, New York 1979. Furthermore, computer simulations have indicated that Gly polymers lack secondary structure and are likely to form a random coil in solution; see Shental-Bechor (2005) Biophys J 88:2391-402. From a chemical perspective, polyglycine is a linear unbranched polyamide that shows certain resemblance to the polyether PEG in so far as both are essentially one-dimensional macromolecules with many rotational degrees of freedom along the chain, which are made of repeated short hydrocarbon units that are regularly interrupted by hydrogen-bonding and highly solvated polar groups. Consequently, polyglycine should constitute the simplest genetically encodable PEG mimetic with prospects for extending the plasma half-life of therapeutic proteins. This concept was employed in form of “homo-amino-acid polymer (HAP)” or as glycine rich sequence (GRS), respectively; see, Schlapschy (2007) Protein Eng Des Sel 20:273-84; WO 2007/103515. However, it has long been known that chemically synthesized pure polymers of Gly show poor solubility in water; see, inter alia, in Bamford C H et al. Synthetic Polypeptides—Preparation, Structure, and Properties. Academic Press, New York 1956. Hence, different attempts were made to increase hydrophilicity, either by introducing hydrogen-bonding serine alcohol side chains (WO 2007/103515 as well as Schlapschy (2007) loc. cit.) or, in addition, negatively charged glutamate residues (WO 2007/103515). It is of note that peptide spacers with the composition (Gly₄Ser)_(n) have already been described in the art in order to link domains in fusion proteins in a flexible manner. A significantly increased hydrodynamic volume was detected for these fusion proteins in analytical SEC. In the case of the 200 residue HAP version the apparent size increase was 120% compared with the unfused Fab fragment, while the true mass was only bigger by 29%, hence revealing the effect of an enhanced hydrodynamic volume due to the solvated random coil structure of the polyglycine tag. Furthermore, CD difference spectra were characteristic for disordered secondary structure for the HAP moiety. Finally, terminal plasma half-life of the Fab fragment carrying the 200 residue HAP in mice was prolonged by approximately a factor 3. Though moderate, this effect could be appropriate for certain (specialized) diagnostic applications, such as in vivo imaging; see Schlapschy (2007); loc. cit. Unfortunately, the production of fusion proteins with longer (Gly₄Ser)_(n) repeat sequences appeared less feasible due to an increasing tendency to form aggregates, thus posing a natural limitation to the use of—more or less pure—glycine polymers as PEG mimetics.

WO 2008/155134 discloses that sequences with an appropriate mixture of Pro, Ala, and Ser (i.e. PAS) residues lead to mutual cancellation of their distinct secondary structure preferences and, thus, result in a stably disordered polypeptide. However, WO 2008/155134 also documents that fusion proteins with a domain composed only of serine and alanine (SA) residues, i.e. a domain comprising only two types of amino acids, do not form a random coil, but a β-sheet structure instead.

The chemical synthesis of polypeptides is well known and has been described in the art. Izuka discloses the chemical synthesis of polypeptides containing proline (see Izuka (1993), Bull. Chem. Soc. Jpn 66, 1269-1272). These copolypeptides contain random sequences of proline and either glycine, L-alanine, L-α-aminobutyric acid (Abu), L-norvaline (Nva) or L-leucine, respectively, and are synthesized by chemical copolymerization. Izuka discloses that such copolypeptides mostly have a defined collagen-like conformation. Further, it is described in this publication that copolypeptides of proline and alanine (or proline and L-a-aminobutyric acid) are partially soluble in water, while other copolypeptides were completely insoluble. It is speculated in Izuka that proline/alanine copolypeptides may have a partial disordered conformation. Izuka emphasizes that chemically synthesized polypeptides with a random proline/alanine sequence occur predominantly in a collagen-like conformation, i.e. in a structured conformation.

Thus, the technical problem underlying the present invention is the provision of large polypeptides with true random coil conformation. The technical problem is solved by provision of the embodiments characterized in the claims and as provided herein.

Accordingly, the invention relates to the provision and use of a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting of at least about 50, in particular of at least about 100, in particular of at least about 150, in particular of at least about 200, in particular of at least about 250, in particular of at least about 300, in particular of at least about 350, in particular of at least about 400 proline and alanine amino acid residues. The invention therefore relates to the provision of biosynthetic random coil polypeptides or polypeptide segments comprising an amino acid sequence of at least 50 amino acid residues, said amino acid sequence consisting solely of proline and alanine amino acid residues and comprising at least one proline and at least one alanine. The invention also provides for a drug conjugate comprising (i) a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, and (ii) a drug selected from the group consisting of (a) a biologically active protein or a polypeptide that comprises or that is an amino acid sequence that has or mediates a biological activity and (b) a small molecule drug. The polypeptides with true random coil conformation and polypeptide segments with true random coil conformation as provided herein are also useful in the context of cosmetic uses as well as uses in food industry and the production of beverages. The large polypeptides provided herein which show true random coil confirmation consist soley and merely of proline (P, Pro) and alanine (A, Ala) residues and comprise more than at least 50 amino acids, in particular of at least about 100, in particular of at least about 150, in particular of at least about 200, in particular of at least about 250, in particular of at least about 300, in particular of at least about 350, in particular of at least about 400 proline and alanine amino acid residues. Both amino acids, P and A, need to be present in the herein provided large polypeptides with true random coil conformation and polypeptide segments with true random coil conformation. Also provided herein are nucleic acid molecules that encode for the herein disclosed biosynthetic random coil polypeptides or polypeptide segments as well as for drug or food conjugates that comprise said biosynthetic random coil polypeptides or polypeptide segments and a (covalently linked) protein of interest, like a biologically active protein.

The biosynthetic random coil polypeptide or biosynthetic random coil polypeptide segment as described herein and to be used in drug or food conjugates as provided herein and comprising an amino acid sequence consisting of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 proline (P) and alanine (A) amino acid residues is, inter alia, to be used in a heterologous context, i.e. in a biologically active heterologous protein, protein construct and/or in a drug conjugate comprising said biosynthetic random coil polypeptide or polypeptide segment and pharmaceutically or medically useful molecules, like small molecules, peptides or biomacromolecules such as proteins, nucleic acids, carbohydrates, lipid vesicles and the like. As illustrated in the appended examples, the inventors could successfully provide for drug conjugates which consist of the true random coil polypeptides as defined herein and biologically active proteins or protein stretches as well as drug conjugates that consist of small molecules or small molecule drugs that comprise and/or are linked to the herein described random coil polypeptides, consisting solely of proline and alanine amino acid residues (i.e. of both amino acids P and A)

Accordingly, the present invention provides, inter alia, for a biologically active, heterologous protein comprising at least two domains wherein (a) a first domain of said at least two domains comprises an amino acid sequence having and/or mediating said biological activity; and (b) a second domain of said at least two domains comprises the biosynthetic random coil polypeptide or polypeptide segment consisting of an amino acid sequence consisting of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 proline and alanine amino acid residues. In accordance with this invention, said “first domain and said “second domain” are not comprised in either a natural (i.e. occurring in nature) protein or a hypothetical protein as deduced from naturally occurring coding nucleic acid sequences, like open reading frames etc.

Furthermore, this invention provides for a drug conjugate consisting of the biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 proline and alanine amino acid residues and (a) pharmaceutically, therapeutically and/or medically useful molecule(s), like (a) small molecule(s), (a) peptide(s) or (a) biomacromolecule(s) such as protein(s), a nucleic acid(s), (a) carbohydrate(s), (a) lipid vesicle(s) and the like, that is/are conjugated to said biosynthetic random coil polypeptide or polypeptide segment. Again, it is of note that the term “biologically active” in context of herein disclosed conjugates is not limited to pure biological molecules but also comprise medically active, therapeutically active, pharmaceutically active molecules and the like. It is evident for the skilled artisan that the means and methods provided herein are not limited to pharmaceutical and medical uses, but can be employed in a wide variety of technologies, including, but not limited to cosmetic, food, beverage and nutrition technologies, oil industry, paper industry and the like.

In contrast to chemically synthesized copolypeptides (like in Izuka, loc.cit.), the random coil polypeptides provided herein are biosynthetically produced. The term “biosynthetic” as used herein refers to the synthesis by means of biotechnological methods (in contrast to chemical synthesis). Such biotechnological methods are well known in the art and also described herein further below. The biosynthesis of the random coil polypeptides of the present invention allows the production of polypeptides with a defined sequence of proline and alanine residues, a defined length and/or a defined ratio of proline and alanine residues. Further, the polypeptides provided in accordance with the present invention are substantially pure, i.e. the produced polypeptides are essentially uniform and share the above characteristics (i.e. defined sequence, defined length and/or defined amino acid ratio). The random coil polypeptides consisting of at least about 50, in particular of at least about 100, in particular of at least about 150, in particular of at least about 200, in particular of at least about 250, in particular of at least about 300, in particular of at least about 350, in particular of at least about 400 proline and alanine amino acid residues are, in accordance with this invention for example comprised in biologically active, heterologous polypeptides/polypeptide constructs and/or in drug or food conjugates as well as in other conjugates useful in further industrial areas, like, but not limited to paper industry, oil industry and the like.

Overall, the above features of the polypeptides of the present invention permit the formation of a stable random coil of the polypeptides and these random coil polypeptides have surprising and advantageous properties. For example, the polypeptides of the present invention are completely soluble in aqueous solution and have an increased hydrodynamic volume. Unexpectedly, the random coil polypeptides as defined herein are also capable of conferring an increased in vivo/in vitro stability. This is particularly important for medical applications, for example, for biologically active proteins or drug conjugates comprising the random coil polypeptide of this invention. However, the numerous advantageous properties of the random coil polypeptides of the present invention not only permit their use in the medical field but also in other fields, like in cosmetics/cosmetic treatments or in the fields of nutrition and food technology, like in the dairy industry or in meat processing. Examples of conjugates useful in food industry and the like are conjugates that comprise the herein disclosed random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues and compounds that are useful in these technologies, like, e.g. polyoxypropylene or polyoxyethylene polymers, which are non-ionic surfactants used as emulsifiers. Also envisaged herein is the use of the biosynthetic random coil polypeptide as defined herein in biochemical methods and in technical processes, such as paper production, oil recovery and the like. The surprising and advantageous characteristics of the biosynthetic random coil polypeptides consisting merely of proline and alanine residues as provided herein (and as also of the herein disclosed conjugates and constructs, like drug or food conjugates/constructs, comprising said biosynthetic, true random coil polypeptides) are described below in greater detail. Furthermore, illustrative uses and means and methods employing these inventive biosynthetic random coil polypeptides are provided below. Also means and methods for the production of such biosynthetic random coil polypeptides as well as biologically active, heterologous polypeptides or polypeptide constructs and of the herein disclosed conjugates and constructs, like drug constructs, comprising said random coil polypeptides are provided herein.

In context of this invention, it has been surprisingly found that proline-alanine polymers/polypeptides with a uniform composition form stable random coil conformation. This is also demonstrated in the appended examples, where random coil structure of biosynthetic proline/alanine (co)-polymers/polypeptides is confirmed by circular dichroism (CD) spectroscopy. Obtaining and employing such biosynthetic, truly random coil polypeptides/polymers was surprising since the established Chou-Fasman method (Chou and Fasman (1974), Biochemistry 13, 223-245) predicts a 100% a-helical secondary structure of polymers/polypeptides (or segments thereof) composed of proline and alanine, as shown in FIG. 7. Yet, herein it has been surprisingly found and experimentally shown that proline-alanine polymers/polypeptides with a uniform composition form a stable random coil conformation. This is also demonstrated in the appended examples, where random coil structure of proline/alanine (co)-polymers/polypeptides is confirmed by experimental techniques like circular dichroism (CD) spectroscopy and size exclusion chromatography (SEC).

In contrast to the polypeptides/polymers of the present invention, the chemically synthesized polypeptides described, for example, in Izuka (1993), loc. cit. have an arbitrary/undefined and stochastic sequence and a diverse length. Thus, the chemically synthesized polypeptides comprise a mixture of completely different peptides with various proline/alanine ratios, lengths, and so on. As mentioned in Izuka, the chemically synthesized polypeptides of such a mixture do not (or only partially) form a random coil and, accordingly, do not have any of the advantageous properties of the biosynthetic polypeptides provided and described herein below. Accordingly, the present invention comprises and relates to compositions comprising the inventive biosynthetic random coil polypeptides/polymers as disclosed herein, whereby said biosynthetic random coil polypeptides/polymers are defined, inter alia, by their sequence comprising solely proline and alanine residues. In one particular embodiment, the present invention relates to conjugates, like drug or food conjugates comprising, as one constituent, these random coil polypeptides/polymers disclosed herein. These inventive biosynthetic random coil polypeptides/polymers comprised in said compositions are, in one embodiment, of uniform length.

As mentioned above, the biosynthetic random coil polypeptides (or random coil polypeptide segments) of this invention consisting solely of proline and alanine residues unexpectedly form a stable random coil conformation. The term “random coil” as used herein relates generally to any conformation of a polymeric molecule, including amino acid polymers/amino acid sequences/polypeptides, in which the individual monomeric elements that form said polymeric structure are essentially randomly oriented towards the adjacent monomeric elements while still being chemically bound to said adjacent monomeric elements. In particular, a polypeptide, amino acid sequence or amino acid polymer adopting/having/forming “random coil conformation” substantially lacks a defined secondary and tertiary structure. In context of the polypeptides of the present invention, the monomeric elements forming the polymeric structure (i.e. the polypeptide/amino acid sequence) are either single amino acids such as proline and alanine per se or peptide stretches such as the “amino acid repeats”/“amino acid cassettes”/“cassette repeats”/“building blocks”/“modules” (or fragments thereof) which are described and defined further below.

The nature of polypeptide random coils and their methods of experimental identification are known to the person skilled in the art and have been described in the scientific literature (Cantor (1980) Biophysical Chemistry, 2nd ed., W. H. Freeman and Company, New York; Creighton (1993) Proteins—Structures and Molecular Properties, 2nd ed., W. H. Freeman and Company, New York; Smith (1996) Fold Des 1:R95-R106). The term “segment” as used herein refers to a part of the herein defined biosynthetic random coil polypeptide, whereby such a part may be an internal part of the biosynthetic random coil polypeptide described herein. Such a “segment” may be, for example, a biosynthetic random coil polypeptide as defined herein where one (or more) amino acid(s) has/have been deleted, e.g. from the start and/or from the end of the polypeptide of the invention. Furthermore, such a “segment” may be used as or may form part of a larger protein or polypeptide, for example, of a fusion protein with a biologically active protein. Such a “fusion protein” would also be an example of a heterologous, biologically active polypeptide/protein/polypeptide construct of the present invention. The term “heterologous” as used herein is defined herein below.

The random coil polypeptide (or random coil segment thereof), as provided in the present invention and to be employed in context of this invention, adopts/forms random coil conformation, for example, in aqueous solution or at physiological conditions. The term “physiological conditions” is known in the art and relates to those conditions in which proteins usually adopt their native, folded conformation. More specifically, the term “physiological conditions” relates to the biophysical parameters as they are typically valid for higher forms of life and, particularly, in mammals, most preferably human beings. The term “physiological conditions” may relate to the biochemical and biophysical parameters as they are normally found in the body (in particular in body fluids) of mammals and in particular in humans. Said “physiological conditions” may relate to the corresponding parameters found in the healthy body as well as the parameters found under disease conditions or in human patients. For example, a sick mammal or human patient may have a higher, yet “physiological” temperature condition when said mammal or said human suffers from fever. With respect to “physiological conditions” at which proteins adopt their native conformation/state, the most important parameters are temperature (37° C. for the human body), pH (7.35-7.45 for human blood), osmolarity (280-300 mmol/kg H₂O), and, if necessary, protein content (66-85 g/l serum). Yet, the person skilled in the art is aware that at physiological conditions these parameters may vary, e.g. the temperature, pH, osmolarity, and protein content may be different in given body or tissue fluids such as blood, liquor cerebrospinalis, peritoneal fluid and lymph (Klinke (2005) Physiologie, 5th ed., Georg Thieme Verlag, Stuttgart). For example, in the liquor cerebrospinalis the osmolarity may be around 290 mmol/kg H₂O and the protein concentration may be between 0.15 g/l to 0.45 g/l while in the lymph the pH may be around 7.4 and the protein content may be between 3 g/l and 5 g/l. When determining whether a polypeptide (or segment thereof)/amino acid sequence forms/adopts random coil conformation under experimental conditions using the methods as described herein below, the biophysical parameters such as temperature, pH, osmolarity and protein content may be different to the physiological conditions normally found in vivo. Temperatures between 1° C. and 42° C. or preferably 4° C. to 25° C. may be considered useful to test and/or verify the biophysical properties and biological activity of a protein under physiological conditions in vitro.

Several buffers, in particular in experimental settings (for example in the determination of protein structures, in particular in CD measurements and other methods that allow the person skilled in the art to determine the structural properties of a protein/amino acid stretch) or in buffers, solvents and/or excipients for pharmaceutical compositions, are considered to represent “physiological solutions”/“physiological conditions” in vitro. Examples of such buffers are, e.g. phosphate-buffered saline (PBS: 115 mM NaCl, 4 mM KH₂PO₄, 16 mM Na₂HPO₄ pH 7.4), Tris buffers, acetate buffers, citrate buffers or similar buffers such as those used in the appended examples. Generally, the pH of a buffer representing “physiological solution conditions” should lie in a range from 6.5 to 8.5, preferably in a range from 7.0 to 8.0, most preferably in a range from 7.2 to 7.7 and the osmolarity should lie in a range from 10 to 1000 mmol/kg H₂O, more preferably in a range from 50 to 500 mmol/kg H₂O and most preferably in a range from 200 to 350 mmol/kg H₂O. Optionally, the protein content of a buffer representing physiological solution conditions may lie in a range from 0 to 100 g/l, neglecting the protein with biological activity itself, whereby typical stabilizing proteins may be used, for example human or bovine serum albumin.

It has been found herein that the polypeptides (or segments thereof) not only form random coil conformation under physiological conditions but, more generally, in aqueous solution. The term “aqueous solution” is well known in the art. An “aqueous solution” may be a solution with a water (H₂O) content of at least about 20%, of at least about 30%, of at least about 40%, of at least about 50%, of at least about 60%, of at least about 70%, of at least about 80% or of at least about 90% H₂O (weight/weight). Accordingly, the polypeptide (or segment thereof) of the present invention may form random coil conformation in aqueous solution, possibly containing other miscible solvents, or in aqueous dispersions with a wider range of temperatures, pH values, osmolarities or protein content. This is particularly relevant for applications of the random coil polypeptide (or segment thereof) outside medical therapy or in vivo diagnostics, for example in cosmetics, nutrition or food technology.

Accordingly, it is also envisaged in the context of this invention that the random coil conformation of the proline/alanine biosynthetic polypeptide (or segment thereof) of the present invention is maintained in and/or is used in context of pharmaceutical compositions, like liquid pharmaceuticals/biologicals or lyophilized pharmaceutical compositions. This is particularly important in context of the herein provided biologically active, heterologous proteins or the drug conjugates comprising, inter alia, the inventive random coil polypeptide (or polypeptide segment). Preferably, “physiological conditions” are to be used in corresponding buffer systems, solvents and/or excipients. Yet, for example in lyophilized or dried compositions (like, e.g. pharmaceutical compositions/biologicals), it is envisaged that the random coil conformation of the herein provided random coil polypeptide (or polypeptide segment) is transiently not present and/or cannot be detected. However, said random coil polypeptide (or polypeptide segment) will adopt/form again its random coil after reconstitution in corresponding buffers/solutions/excipients/solvents or after administration to the body. Methods for determining whether a polypeptide (or segment thereof) forms/adopts random coil conformation are known in the art (Cantor (1980) loc. cit.; Creighton (1993) loc. cit.; Smith (1996) loc. cit.). Such methods include circular dichroism (CD) spectroscopy as exemplified herein below. CD spectroscopy represents a light absorption spectroscopy method in which the difference in absorbance of right- and left-circularly polarized light by a substance is measured. The secondary structure of a protein can be determined by CD spectroscopy using far-ultraviolet spectra with a wavelength between approximately 190 and 250 nm. At these wavelengths, the different secondary structures commonly found in polypeptides can be analyzed, since α-helix, parallel and anti-parallel β-sheet, and random coil conformations each give rise to a characteristic shape and magnitude of the CD spectrum. Accordingly, by using CD spectrometry the skilled artisan is readily capable of determining whether polypeptide (or segment thereof) forms/adopts random coil conformation in aqueous solution or at physiological conditions. Other established biophysical methods include nuclear magnetic resonance (NMR) spectroscopy, absorption spectrometry, infrared and Raman spectroscopy, measurement of the hydrodynamic volume via size exclusion chromatography, analytical ultracentrifugation or dynamic/static light scattering as well as measurements of the frictional coefficient or intrinsic viscosity (Cantor (1980) loc. cit.; Creighton (1993) loc. cit.; Smith (1996) loc. cit.).

In addition to the experimental methods above, theoretical methods for the prediction of secondary structures in proteins have been described. One example of such a theoretical method is the Chou-Fasman method (Chou and Fasman, loc.cit.) which is based on an analysis of the relative frequencies of each amino acid in α-helices, β-sheets, and turns based on known protein structures solved, for example, with X-ray crystallography. However, theoretical prediction of protein secondary structure is known to be unreliable. As exemplified herein below, amino acid sequences expected to adopt an a-helical secondary structure according to the Chou-Fasman method were experimentally found to form a random coil. Accordingly, theoretical methods such as the Chou-Fasman algorithm may only have limited predictive value whether a given polypeptide adopts random coil conformation, as also illustrated in the appended examples and figures. Nonetheless, the above described theoretical prediction is often the first approach in the evaluation of a putative secondary structure of a given polypeptide/amino acid sequence. A theoretical prediction of a random coil structure also often indicates that it might be worthwhile verifying by the above experimental means whether a given polypeptide/amino acid sequence has indeed a random coil conformation.

Homo-polymers of most amino acids, in particular the hydrophobic amino acids, are usually insoluble in aqueous solution (Bamford (1956) Synthetic Polypeptides—Preparation, Structure, and Properties, 2nd ed., Academic Press, New York). Homo-polymers of several hydrophilic amino acids are known to form secondary structures, for example α-helix in the case of Ala (Shental-Bechor (2005) Biophys J 88:2391-2402) and β-sheet in the case of Ser (Quadrifoglio (1968) J Am Chem Soc 90:2760-2765) while poly-proline, the stiffest homooligopeptide (Schimmel (1967) Proc Natl Acad Sci USA 58:52-59), forms a type II trans helix in aqueous solution (Cowan (1955) Nature 176:501-503).

Using the theoretical principles of polymer biophysics the random coil diameter of a chain of 200 amino acid residues would amount in the case of poly-glycine, for example, to ca. 75 Å—calculated as the average root mean square end-to-end distance of

=I·√{square root over (n·C_(∞))}, with n=200 rotatable bonds of length 1=3.8 Å for each Cα-Cα distance and the ‘characteristic ratio’ C_(∞)≈2.0 for poly(Gly) (Brant (1967) J Mol Biol 23:47-65; Creighton, (1993) loc.cit.). This relation shows that the person skilled in the art would expect that the hydrodynamic volume of a random chain amino acid polymer can be either extended by (a) using a longer chain length 1 or by (b) using amino acids that exhibit a larger characteristic ratio, C_(∞). C_(∞) is a measure for the inherent stiffness of the molecular random chain and has a general value of 9 for most amino acids (Brant (1967) loc.cit.). Only Gly, which lacks a side chain, and also the imino acid Pro exhibit significantly smaller values. Hence, Gly and Pro (under denaturing conditions) are expected to contribute to reducing the dimensions of random coil proteins (Miller (1968) Biochemistry 7:3925-3935). Amino acid sequences comprising proline residues, accordingly, are expected to have a relatively compact hydrodynamic volume. In contrast to this teaching, however, it is shown herein that the hydrodynamic volume of the amino acid polymers/polypeptides of the invention that comprise a mixture of proline and alanine residues have a dramatically increased hydrodynamic volume as determined by analytical gel permeation/size exclusion chromatography when compared to the expected hydrodynamic volume. In fact, it is surprising that polypeptides comprising mixtures of these two amino acids (proline and alanine), of which each alone tends to form a homooligopeptide with defined secondary structure, adopt random coil conformation under physiological conditions. Such inventive proline/alanine polypeptides have a larger hydrodynamic radius than homo-polymers comprising the same number of Gly residues, for example, and they confer better solubility to the biologically active proteins or constructs, i.e. biologically active heterologous proteins or drug conjugates, according to the invention.

As mentioned above, the biosynthetic random coil proline/alanine polypeptides of the present invention differ from chemically synthesized polypeptides in that they can adopt a defined, uniform length by easy means and methods. Whereas the prior art provides mixtures/compositions of polypeptides with enormous variations in terms of the length of the peptides, the present invention can provide mixtures/compositions of biosynthetic random coil polypeptides with a defined length. Preferably, essentially all polypeptides of the invention comprised in such a mixture/composition have the same defined length, and, hence, share the same biochemical characteristics. Such a uniform composition is more advantageous in the various medical, cosmetic, nutritional applications, wherein the biosynthetic random coil polypeptides can be employed. Furthermore, in particular in a medical or pharmaceutical context, the herein defined biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting of at least about 50, in particular of at least about 100, in particular of at least about 150, in particular of at least about 200, in particular of at least about 250, in particular of at least about 300, in particular of at least about 350, in particular of at least about 400 proline and alanine amino acid residues can also be used in the prevention, amelioration and/or treatment of disorders linked and/or affiliated with an impaired blood plasma situation, for example after injuries, burns, surgery and the like. One medical use of said biosynthetic random coil polypeptides or polypeptide segments is, accordingly, the use as plasma expander. However, it is of note that in accordance with this invention also the herein described drug conjugates and heterologous polypeptides or heterologous polypeptide constructs may be employed in context of the medical or pharmaceutical intervention of a disorder related to an impaired blood plasma amount or blood plasma content or of a disorder related to an impaired blood volume.

Accordingly, the present invention relates in one embodiment to a biosynthetic random polypeptide (or segment thereof) which comprises an amino acid sequence consisting solely of at least about 50 proline and alanine amino acid residues, of at least about 100 proline and alanine amino acid residues, of at least about 150 proline and alanine amino acid residues or of at least about 200 proline and alanine residues, in particular when comprised in a heterologous protein/polypeptide/polypeptide construct or in a drug conjugate. The present invention also relates to biosynthetic random coil polypeptides which comprise an amino acid sequence consisting solely of at least about 200 proline and alanine amino acid residues, even more preferably of at least about 300 proline and alanine amino acid residues, particularly preferably of at least about 400 proline and alanine amino acid residues, more particularly preferably of at least about 500 proline and alanine amino acid residues and most preferably of at least about 600 proline and alanine amino acid residues. The amino acid sequence forming random coil conformation may consist of maximally about 3000 proline and alanine amino acid residues, of maximally about 2000 proline and alanine amino acid residues, of maximally about 1500 proline and alanine amino acid residues, of maximally about 1200 proline and alanine amino acid residues, of maximally about 800 proline and alanine amino acid residues. Accordingly, the proline/alanine amino acid sequence stretch may consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400, of about 500, of about 600, of about 700, of about 800, of about 900 to about 3000 proline and alanine amino acid residues. In certain embodiments, the inventive biosynthetic amino acid sequence comprises about 200 to about 3000 proline and alanine residues, about 200 to about 2500 proline and alanine residues, about 200 to about 2000 proline and alanine residues, about 200 to about 1500 proline and alanine residues, about 200 to about 1000 proline and alanine residues, about 300 to about 3000 proline and alanine residues, about 300 to about 2500 proline and alanine residues, about 300 to about 2000 proline and alanine residues, about 300 to about 1500 proline and alanine residues, about 300 to about 1000 proline and alanine residues, about 400 to about 3000 proline and alanine residues, about 400 to about 2500 proline and alanine residues, about 400 to about 2000 proline and alanine residues, about 400 to about 1500 proline and alanine residues, about 400 to about 1000 proline and alanine residues, about 500 to about 3000 proline and alanine residues, about 500 to about 2500 proline and alanine residues, about 500 to about 2000 proline and alanine residues, about 500 to about 1500 proline and alanine residues, about 500 to about 1000 proline and alanine residues, about 600 to about 3000 proline and alanine residues, about 600 to about 2500 proline and alanine residues, about 600 to about 2000 proline and alanine residues, about 600 to about 1500 proline and alanine residues, about 600 to about 1000 proline and alanine residues, about 700 to about 3000 proline and alanine residues, about 700 to about 2500 proline and alanine residues, about 700 to about 2000 proline and alanine residues, about 700 to about 1500 proline and alanine residues, about 700 to about 1000 proline and alanine residues, about 800 to about 3000 proline and alanine residues, about 800 to about 2500 proline and alanine residues, about 800 to about 2000 proline and alanine residues, about 800 to about 1500 proline and alanine residues, about 800 to about 1000 proline and alanine residues. As is evident from the content of this invention, also larger biosynthetic amino acid sequences (consisting essentially of proline and alanine) are within the scope of this invention and can readily be employed in the herein defined biologically active proteins or protein constructs which comprise as one domain of at least two domains an amino acid sequence having and/or mediating said biological activity and as another domain of at least two domains the biosynthetic random coil polypeptide or polypeptide segment consisting of at least about 50 proline and alanine amino acid residues, of at least about 100 proline and alanine amino acid residues, of at least about 150 proline and alanine amino acid residues, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 proline and alanine amino acid residues. Such a biosynthetic random coil polypeptide or polypeptide segment corresponds to the biosynthetic random coil part of a heterologous protein/protein construct. These biosynthetic proline/alanine stretches consist of maximally about 3000 proline and alanine amino acid residues. These amino acid sequences (proline/alanine stretches) comprise proline and alanine as main or unique residues as explained further below.

It is envisaged that it is the herein defined biosynthetic amino acid sequence consisting solely of proline (P) and alanine (A) amino acid residues, which forms/adopts/has a random coil conformation. In the simplest case, the biosynthetic polypeptide or polypeptide segment consists of the amino acid sequence having a random coil conformation as defined herein. However, the biosynthetic polypeptide (or segment thereof) may, in addition to the herein described amino acid sequence forming/adopting/having a random coil conformation, comprise further amino acid sequences/amino acid residues which do not contribute to the formation of the random coil conformation or which are not capable of forming/adopting/having a random coil conformation on their own. Without deferring from the gist of the invention, also such biosynthetic polypeptides (or segments thereof) are biosynthetic “random coil” polypeptides or polypeptide segments. The further amino acid sequences/amino acid residues may, for example, be useful as linkers. Inter alia, dimers, trimers, i.e. in general multimers of the biosynthetic random coil polypeptide are also envisaged in context of the present invention and such multimers may be linked by amino acid sequences/residues which do not form random coil conformation. An example of a protein which may comprise such a random coil polypeptide is the herein provided biologically active protein, which may, in addition to the random coil polypeptide consisting of proline and alanine amino acid residues as defined herein further comprise another polypeptide having/mediating biological activity. Again, such a construct may be a heterologous, biologically active protein or polypeptide construct as described herein.

The term “at least about 50/100/150/200/300/400/500/600/700/800/etc. amino acid residues” is not limited to the concise number of amino acid residues but also comprises amino acid stretches that comprise either additional about 1-20%, like 10% to 20% residues or about 1-20%, like about 10% to 20% less residues. For example “at least about 100 amino acid residues” may also comprise about 80 to 100 and about 100 to 120 amino acid residues without deferring from the gist of the present invention. For example “at least about 200 amino acid residues” may also comprise about 160 to 200 and about 200 to 240 amino acid residues without deferring from the gist of this invention. The definition and explanations given herein above, apply, mutatis mutandis, also to the term “maximally about 3000/2000/1500/1200/800 amino acid residues” etc. Accordingly, the term “about” is not limited or restricted to the concise number of amino acid residues in context of longer amino acid sequences (e.g. amino acid sequences comprising or consisting of maximally 3000 amino acid residues). Therefore, the term “maximally about 3000/2000/1500/1200/800 amino acid residues” but may also comprise amino acid stretches that comprise additional 10% to 20% or 10% to 20% less residues without deferring from this invention.

Furthermore, the biosynthetic random coil polypeptides (or segments thereof) are characterised by a defined content or ratio of amino acid residues, in particular of the main constituents proline and alanine. As mentioned above, the present invention relates to a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least about 50, of at least about 100, of at least about 150, of at least about 200 of at least about 250, of at least about 300, of at least about 350, of at least about 400 proline (Pro) and alanine (Ala) amino acid residues in particular when comprised in a heterologous biological active protein/protein construct/polypeptide or drug conjugate. The term “solely” as used herein means that preferably at least about 90% or at least about 95% of the amino acids are proline and alanine, whereby proline and alanine constitute the majority but may not be the only amino acid residues, i.e. these inventive amino acid sequences are not necessarily 100% proline and alanine amino acid stretches. Hence, the biosynthetic polypeptides/amino acid sequences of the present invention may also comprise other amino acids than proline and alanine as minor constituents as long as the amino acid sequence forms/adopts/has random coil conformation. Such a random coil conformation can be easily determined by herein provided means and methods. Accordingly, also in context of the term “solely”, a minor amount (less than about 10% or less than about 5%) of other amino acid residues may be comprised. Said “other”, minor amino acid residues are defined herein below.

Accordingly, the present invention relates in one embodiment to a biosynthetic random coil polypeptide (or segment thereof) whereby the amino acid sequence consists mainly of proline and alanine, and wherein the proline residues constitute more than about 10% and less than 75% of the amino acid sequence. The alanine residues comprise the remaining at least 25% to 90% of said amino acid sequence (or the random coil polypeptide or polypeptide segment if it consists of the amino acid sequence).

Preferably, the amino acid sequence comprises more than about 10%, preferably more than about 12%, even more preferably more than about 14%, particularly preferably more than about 18%, more particularly preferably more than about 20%, even more particularly preferably more than about 22%, 23% or 24% and most preferably more than about 25% proline residues. The amino acid sequence preferably comprises less than about 75%, more preferably less than 70%, 65%, 60%, 55% or 50% proline residues, wherein the lower values are preferred. Even more preferably, the amino acid sequence comprises less than about 48%, 46%, 44%, 42% proline residues. Particular preferred are amino acid sequences comprising less than about 41%, 40%, 39% 38%, 37% or 36% proline residues, whereby lower values are preferred. Most preferably, the amino acid sequence comprise less than about 35% proline residues; see also the herein below provided PA constructs.

Vice versa, the amino acid sequence preferably comprises less than about 90%, more preferably less than 88%, 86%, 84%, 82% or 80% alanine residues, wherein the lower values are preferred. Even more preferably, the amino acid sequence comprises less than about 79%, 78%, 77%, 76% alanine residues, whereby lower values are preferred. Most preferably, the amino acid sequence comprises less than about 75% alanine residues.

Also preferred herein is an amino acid sequence comprising more than about 25%, preferably more than about 30%, even more preferably more than about 35%, particularly preferably more than about 40%, more particularly preferably more than about 45% or 50%, even more particularly preferably more than about 52%, 54%, 56%, 58% or 59% alanine residues, wherein the higher values are preferred. Even more preferably, the amino acid sequence comprises more than about 60%, 61%, 62%, 63% or 64% alanine residues and most preferably more than about 65% alanine residues.

Accordingly, the random coil polypeptide (or segment thereof) may comprise an amino acid sequence consisting of about 25% proline residues, and about 75% alanine residues. Alternatively, the random coil polypeptide (or segment thereof) may comprise an amino acid sequence consisting of about 35% proline residues and about 65% alanine residues. The term “about X %” as used herein above is not limited to the concise number of the percentage, but also comprises values of additional 10% to 20% or 10% to 20% less residues. For example the term 10% may also relate to 11% or 12% and to 9% and 8%, respectively.

However, as mentioned above and further detailed herein below said random coil polypeptide (or polypeptide segment), and, in particular the amino acid sequence, may also comprise additional amino acids differing from proline and alanine as minor constituents. As already discussed herein above, said minor constituent(s), i.e. (an)other amino acid(s) than proline or alanine, may comprise less than about 10%, less than about 9%, less than about 8%, less than about 7%, less than about 6%, less than about 5%, less than about 4%, less than about 4%, less than about 3% or less than about 2% of the biosynthetic random coil polypeptide/polymer of this invention.

The skilled person is aware that an amino acid sequence/polypeptide (or segment thereof) may also form random coil conformation when other residues than proline and alanine are comprised as a minor constituent in said amino acid sequence/polypeptide (polypeptide segment). The term “minor constituent” as used herein means that maximally 5% or maximally 10% amino acid residues are different from proline or alanine in the inventive biosynthetic random coil polypeptides/polymers of this invention.—This means that maximally 10 of 100 amino acids may be different from proline and alanine, preferably maximally 8%, i.e. maximally 8 of 100 amino acids may be different from proline and alanine, more preferably maximally 6%, i.e. maximally 6 of 100 amino acids may be different from proline and alanine, even more preferably maximally 5%, i.e. maximally 5 of 100 amino acids may be different from proline and alanine, particularly preferably maximally 4%, i.e. maximally 4 of 100 amino acids may be different from proline and alanine, more particularly preferably maximally 3%, i.e. maximally 3 of 100 amino acids may be different from proline and alanine, even more particularly preferably maximally 2%, i.e. maximally 2 of 100 amino acids may be different from proline and alanine and most preferably maximally 1%, i.e. maximally 1 of 100 of the amino acids that are comprised in the random coil polypeptide (or segment thereof) may be different from proline and alanine. Said amino acids different from proline and alanine, may be selected from the group consisting of Arg, Asn, Asp, Cys, Gln, Glu, Gly, His, Ile, Leu, Lys, Met, Phe, Thr, Trp, Tyr, and Val, including posttranslationally modified amino acids or non-natural amino acids (see, e.g., Budisa (2004) Angew Chem Int Ed Engl 43:6426-6463 or Young (2010) J Biol Chem 285:11039-11044). In case that the “minor constituent” (i.e. an amino acid other than proline and alanine) of the biosynthetic random coil polypeptide/construct/polymer (or a fragment thereof) comprises as “other amino acid”/“different amino acid” (a) Ser(s), said Ser amino acid/Ser amino acids constitute preferably less than 50%, more preferably less than 40%, less than 30%, less than 20% or less than 10% of these (minor) amino acid residues. In a most preferred embodiment, the biosynthetic random coil polypeptide/construct/polymer as described herein or the random coil polypeptide part of a (e.g.) fusion protein as described herein does not comprise (a) serine residue(s). It is, generally, preferred herein that these “minor” amino acids (other than proline and alanine) are not present in the herein provided biosynthetic random coil polypeptide/construct/polymer as described herein or the random coil polypeptide part of a (e.g.) fusion protein. In accordance with the invention, a biosynthetic random coil polypeptide (or segment thereof)/the amino acid sequence may, in particular, consist exclusively of proline and alanine amino acid residues (i.e. no other amino acid residues are present in the random coil polypeptide or in the amino acid sequence).

Whereas the above relates to the overall length and proline/alanine content of the amino acid sequence comprised in the random coil polypeptide (or segment thereof), the following relates in greater detail to the specific, exemplary amino acid sequences (or fragments thereof).

In one embodiment, the amino acid sequences/polypeptides adopting random coil conformation (the random coil polypeptide or segment thereof as defined herein), for example, in aqueous solution or under physiological conditions may comprise a plurality of “amino acid repeats”/“amino acid cassettes”/“cassette repeats”, wherein said “amino acid repeats”/“amino acid cassettes”/“cassette repeats”/“building block”/“modules” (these terms are used herein interchangeably) mainly or exclusively consist of proline (Pro, P) and alanine (Ala, A) amino acid residues (depicted herein as “PA”, or as “AP”), wherein no more than 6 consecutive amino acid residues are identical. An illustrative “building block” is, e.g. “AP” and this has also been provided in the appended illustrative examples as functional biosynthetic random coil domain of the present invention. This illustrative example is the sequence “P1A1” as also provided in form of APAPAPAPAPAPAPAPAPAP (SEQ ID NO: 51). i.e. a “poly PA” “amino acid repeat”/“amino acid cassette”/“cassette repeat”. In a preferred embodiment, the amino acid sequence/polypeptide comprising the above defined “amino acid repeats”/“amino acid cassettes”/“cassette repeats” and the like comprises no more than 5 identical consecutive amino acid residues. Other alternative embodiments are provided herein below in context of exemplified, individual building blocks.

Within a random coil polypeptide (or segment thereof) according to this invention the amino acid repeats may be identical or non-identical. Non-limiting examples of “amino acid repeats”, “building blocks”, “modules”, “repeats”, “amino acid cassettes” etc. consisting of proline and alanine residues are provided herein below; see, e.g. SEQ ID NO: 1, SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6 and SEQ ID NO. 51 (The enclosed sequence listing also comprises illustrative nucleic acid sequences which encode such “repeats”/“modules”, etc. The appended sequences in said sequence listing as filed herewith constitute part of this specification and description). Also the use of (identical and/or non-identical) fragments of these sequences is envisasged herein, whereby a “fragment” comprises at least 2 amino acids and comprises at least one proline and/or alanine, preferably at least one proline and one alanine. “Fragments” of these sequences to be employed in accordance with this invention for the generation of the random coil polypeptide (or segment thereof) may consist of at least 3, preferably of at least 4, more preferably of at least 5, even more preferably of at least 6, still more preferably of at least 8, particularly preferably of at least 10, more particularly preferably of at least 12, even more particularly preferably of at least 14, still more particularly preferably of at least 16, and most preferably of at least 18 consecutive amino acids of the amino acid sequence selected from the group consisting of said SEQ ID NOs: 1, 2, 3, 4, 5, 6 and 51 (here it is of note that SEQ ID No. 51 consists of an illustrative “AP” or “PA” repeat).

Based on the teaching given herein, the person skilled in the art is readily in a position to generate further amino acid sequences/polypeptides that form random coil conformation for example under aqueous or under physiological conditions and are constituted of mainly proline and alanine as defined herein. Further examples of random coil conformation forming amino acid sequences/polypeptides to be used as building blocks or modules of the herein defined random coil polypeptide (or segment thereof) may, inter alia, comprise combinations and/or fragments or circularly permuted versions of the specific “building blocks”, “polymer cassettes”, or “polymer repeats” shown above. Accordingly, the exemplified modules/sequence units/polymer repeats/polymer cassettes of the random coil polypeptide/amino acid sequence may also provide for individual fragments which may be newly combined to form further modules/sequence units/polymer repeats/polymer cassettes in accordance with this invention.

The terms “module(s)”, “sequence unit(s)”, “polymer repeat(s)”, “polymer cassette(s)” and “building block(s) are used as synonyms herein and relate to individual amino acid stretches which may be used to form the herein defined random coil polypeptide (or segment thereof)/amino acid sequence.

An amino acid repeat (used as “building block” etc. of a biosynthetic random coil polypeptide of the present invention) may consist of at least 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29, 30 or more amino acid residues, wherein each repeat comprises (an) proline and alanine residue(s). However, as illustrated in appended SEQ ID No. 51, said “building block” can also merely consist of the 2 herein provided amino acid residues P and A, namely in form of “PA” or “AP”. In one embodiment, the amino acid repeat according to the present invention does not comprise more than 50 amino acid residues. However, it is evident for the skilled artisan that such a “repeat” may comprise even more than 50 amino acid residues, for example in cases wherein said inventive biosynthetic random coil polypeptide/polymer comprises more than about, e.g., 100 amino acids, more than about 150 amino acids, more than about 200 amino acids, etc. Accordingly, the maximal amount of amino acid residues comprised in such a “repeat” is conditioned by the over-all length of the biosynthetic polypeptide (or segment thereof)/polymer as provided herein.

Yet, it is of note that the biosynthetic random coil polypeptides/amino acid sequences comprising the above repeats etc. should preferably have the overall length and/or proline/alanine content as defined and explained herein above, i.e. consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 amino acids and/or comprise more than about 10% and less than about 75% proline residues. All the definitions given herein above in this context also apply here, mutatis mutandis.

As discussed in detail herein and as provided herein above, the present invention provides for (a) biologically active, heterologous protein(s) or (a) protein construct(s) that is/are particularly useful in a pharmaceutical, medical and/or medicinal setting. These biologically active, heterologous proteins/protein constructs comprise as at least one domain of said at least two domains the random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine residues, wherein said amino acid sequence consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 proline (Pro) and alanine (Ala) residues.

In context of the biologically active, heterologous proteins, polypeptides or protein constructs as disclosed herein, the term “heterologous” relates to at least two domains within said proteins, polypeptides or protein constructs wherein a first of said at least two domains confers, has and/or mediates a defined biological activity and wherein a second of said at least two domains comprises the biosynthetic random coil polypeptide consisting solely of proline and alanine amino acid residues and whereby said at least two domains are not found operationally linked to each other in nature or are not encoded by a single coding nucleic acid sequence (like an open reading frame) existing in nature. The biosynthetic random coil polypeptide/polypeptide segment consisting solely of proline and alanine amino acid residues as provided herein and as employed in the biologically active, heterologous proteins/protein constructs of this invention are preferably not further (chemically) modified, for example they are preferably neither glycosylated nor hydroxylated.

It is of note that certain naturally occurring proteins or hypothetical proteins as deduced from sequenced nucleic acid stretches found in nature are described as comprising a relatively high (i.e. above average) content of proline and alanine. For example, a homologous hypothetical protein has been described for Leishmania major strain Friedlin (Ivens (2005) Science 309, 436-442.). The disclosed reading frame comprising 1514 codon triplets includes a stretch of 412 triplets composed of 240 Ala, 132 Pro, 34 Lys and 4 Val codons. The Lys residues, which are positively charged under physiological buffer conditions, are almost evenly distributed among this sequence, suggesting a solubilizing effect. However, as is evident from the disclosure herein, such a homologous hypothetical protein as deduced from a naturally occurring nucleic acid molecule or open reading frame, comprising a high proline and alanine content above average is not part of this invention. The invention is based on the fact that a rather large random coil polypeptide or polypeptide segment that does not occur in nature in an isolated manner and that comprises an amino acid sequence consisting solely of proline and alanine residues, wherein said amino acid sequence consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 proline (Pro) and alanine (Ala) residues is provided that is particularly useful in medical/pharmaceutical context. The herein described isolated biosynthetic random coil polypeptides or polypeptide segments that do not occur in nature in an isolated manner are also comprised in the herein disclosed (a) biologically active, heterologous protein(s) or (a) protein construct(s) that is/are particularly useful in a pharmaceutical, medical and/or medicinal setting. These biologically active, heterologous proteins/protein constructs comprise as at least one domain of said at least two domains the random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine residues, wherein said amino acid sequence consists of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 proline (Pro) and alanine (Ala) residues.

Also, arabinogalactan proteins (AGPs), Pro-rich proteins, and extensins belong to a large group of glycoproteins, known as hydroxyproline (Hyp)-rich glycoproteins (HRGPs), which are expressed throughout the plant kingdom. One such AGP motif comprising an Ala-Pro repeat (AP)51 was expressed as a synthetic glycomodule peptide with N-terminal signal sequence and C-terminal green fluorescent protein in transgenic Arabidopsis thaliana and investigated as a substrate for prolyl hydroxylases and subsequent O-glycosylation of the hydroxyproline residues (Estévez (2006) Plant Physiol. 142, 458-470). Again, the disclosed hydroxylated and/or glycosylated Pro side chains, which can form hydrogen bonds to water molecules, appear to have a solubilizing effect.

It is of note that the herein described “biologically active proteins or protein constructs comprising as (at least) one domain a biosynthetic random coil polypeptide or peptide segment comprising an amino acid sequence consisting solely of proline and alanine residues” relate to proteins or protein constructs that do not normally occur in nature and, thus, are “heterologous”. Furthermore, and in contrast to proline-rich sequences described in the plant kingdom, the biosynthetic random coil polypeptides/polypeptide segments described herein are preferably not chemically modified, i.e. they are preferably not glycosylated or hydroxylated.

A particular advantage of the biosynthetic random coil polypeptides or polypeptide segments of this invention is their intrinsically hydrophilic but uncharged character. Accordingly, as “minor” amino acids (other than proline and alanine) in the herein described biosynthetic random coil polypeptide or polypeptide stretch such amino acids are preferred that do not have hydrophobic side chains, like Val, Ile, Leu, Met, Phe, Tyr or Trp, and/or that do not have charged side chains, like Lys, Arg, Asp or Glu. In accordance with this invention, it is envisaged that (in cases where such individual amino acids are nevertheless comprised in the inventive biosynthetic random coil polypeptide/polypeptide segment) the overall content of each individual amino acid having a hydrophobic side chain, like Val, Ile, Leu, Met, Phe, Tyr or Trp, and/or having a charged side chain, like Lys, Arg, Asp, or Glu, within the herein defined biosynthetic random coil polypeptide (or segment thereof) does not exceed 8%, 7%, 6% 5%, 4%, 3%, 2% or 1%.

The biosynthetic random coil polypeptide/amino acid sequences of the present invention may comprise concatamers of individual blocks comprising combined proline/alanine stretches of the sequence (Pro)_(x)-(Ala)_(y), whereby x can have an integer value from 1 to preferably 15, more preferably 1 to 10, even more preferably 1 to 5, and y can have an integer value from 1 to preferably 15, more preferably 1 to 10, even more preferably 1 to 5, and x and y can vary between subsequent blocks. Said x and y can also be an integer of 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14 or 15.

The amino acid sequences/polypeptides forming random coil conformation in aqueous solution or under physiological conditions may have the formula (I): [Pro_(x)Ala_(y)]_(n) wherein x is independently selected from integer 1 to 5. Furthermore, for each n, y is independently selected from integer 1 to 5. n, finally, is any integer provided that random coil polypeptide (or segment thereof)/amino acid sequence consists preferably of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 amino acid residues and up to about 3000 amino acid residues. Also in this context it is of note that the polypeptides/amino acid sequences comprising the above concatemers or having the above formula (I) should preferably have the overall length and/or proline/alanine content as defined and explained herein above, i.e. consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 amino acids and/or comprise more than about 10% and less than about 75% proline residues. Again, all the definitions given herein above in this context also apply here, mutatis mutandis.

The present invention also relates to random coil polypeptides ((a)polypeptide segment(s))/amino acid sequences comprising an amino acid stretch selected from the group consisting of AAPAAPAPAAPAAPAPAAPA (SEQ ID NO: 1); AAPAAAPAPAAPAAPAPAAP (SEQ ID NO: 2); AAAPAAAPAAAPAAAPAAAP (SEQ ID NO: 3 being an example for [Pro₁Ala₃]₅); AAPAAPAAPAAPAAPAAPAAPAAP (SEQ ID NO: 4); APAAAPAPAAAPAPAAAPAPAAAP (SEQ ID NO: 5); AAAPAAPAAPPAAAAPAAPAAPPA (SEQ ID NO: 6) and APAPAPAPAPAPAPAPAPAP (SEQ ID NO: 51 being an example for [Pro₁Ala₁]₁₀) or circular permuted versions or (a) multimers(s) of these sequences as a whole or parts of these sequences. Accordingly, the random coil polypeptide ((a) polypeptide segment(s) thereof)/amino acid sequence may comprise the amino acid stretch AAPAAPAPAAPAAPAPAAPA (SEQ ID NO: 1), AAPAAPAPAAPAAPAPAAPA (SEQ ID NO: 1); AAPAAAPAPAAPAAPAPAAP (SEQ ID NO: 2); AAAPAAAPAAAPAAAPAAAP (SEQ ID NO: 3); AAPAAPAAPAAPAAPAAPAAPAAP (SEQ ID NO: 4); APAAAPAPAAAPAPAAAPAPAAAP (SEQ ID NO: 5); AAAPAAPAAPPAAAAPAAPAAPPA (SEQ ID NO: 6) and APAPAPAPAPAPAPAPAPAP (SEQ ID NO: 51), as well as combinations of these motifs or combinations of fragments and parts of this motifs as long as the resulting biosynthetic random coil polypeptide consists solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues.

Also circular permuted versions of the above amino acid sequences may be used in accordance with the present invention. Exemplary circular permuted versions of e.g. AAPAAPAPAAPAAPAPAAPA (SEQ ID NO: 1) can be easily generated, for example by removing the first alanine and adding another alanine at the end of the above sequence. Such a circular permuted version of SEQ ID NO: 1 would then be APAAPAPAAPAAPAPAAPAA (SEQ ID NO: 7). Further, non-limiting examples of circular permuted versions of SEQ ID NO. 1 are:

(SEQ ID NO: 8) PAAPAPAAPAAPAPAAPAAA, (SEQ ID NO: 9) AAPAPAAPAAPAPAAPAAAP, (SEQ ID NO: 10) APAPAAPAAPAPAAPAAAPA, (SEQ ID NO: 11) PAPAAPAAPAPAAPAAAPAA, (SEQ ID NO: 12) APAAPAAPAPAAPAAAPAAP, (SEQ ID NO: 13) PAAPAAPAPAAPAAAPAAPA, (SEQ ID NO: 14) AAPAAPAPAAPAAAPAAPAP, (SEQ ID NO: 15) APAAPAPAAPAAAPAAPAPA, (SEQ ID NO: 16) PAAPAPAAPAAAPAAPAPAA, and the like. Based on the teaching of the present invention, a skilled person is easily in the position to generate corresponding circular permuted versions of the amino acid stretches as shown in SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6 and SEQ ID NO. 51 (said SEQ ID No. 51 being entirely based on “AP” repeats and a circular permutated version could be based entirely on “PA” or “AP” repeats/building blocks).

Such circular permuted versions may also be considered as examples of a further “module”/“building block” etc. of the herein provided polypeptides/amino acid sequences which can be used accordingly herein.

It is evident for the person skilled in the art that also “modules” and (shorter) fragments or circularly permuted versions of the herein provided amino acid stretches may be used as “modules”, “repeats” and/or building blocks for the herein defined random coil polypeptide (or segment thereof)/amino acid sequence.

In accordance with the above, the random coil polypeptide/amino acid sequence forming random coil conformation may comprise a multimer of any of the above amino acid stretches (or circular permuted versions or fragments thereof), preferably those shown in SEQ ID NO: 1, SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6 and SEQ ID NO. 51. It is to note that these sequences are by no means limiting in context of this invention.

Again, the polypeptides/amino acid sequences comprising the above amino acid stretches (or fragments thereof), circular mutated versions (or fragments thereof) should preferably have the overall length and/or proline/alanine content as defined and explained herein above, i.e. consist of about 50, of about 100, of about 150, of about 200, of about 250, of about 300, of about 350, of about 400 to about 3000 amino acids and/or comprise more than about 10% and less than about 75% proline residues. All the definitions given herein above in this context also apply here, mutatis mutandis. Also the term “fragment” has been defined above.

As mentioned above, in context of this invention it was surprisingly found that the biosynthetic random coil polypeptides (or polypeptide segment)/polymers as provided herein are characterized by a relatively large hydrodynamic volume. This hydrodynamic volume, also called apparent size, can easily be determined by analytical gel filtration (also known as size exclusion chromatography, SEC). Preferably, the random coil polypeptide (or segment thereof) has an apparent size of at least 10 kDa, preferably of at least 25 kDa, more preferably of at least 50 kDa, even more preferably of at least 100 kDa, particularly preferably of at least 200 kDa and most preferably of at least 400 kDa. The person skilled in the art is readily capable of determining the hydrodynamic volume of specific proteins. Such methods may include dynamic/static light scattering, analytical ultracentrifugation or analytical gel filtration as exemplified herein below. Analytical gel filtration represents a known method in the art for measuring the hydrodynamic volume of macromolecules. Alternatively, the hydrodynamic volume of a globular polypeptide can be estimated by its molecular weight (Creighton (1993) loc. cit.). As described herein the hydrodynamic volume of the polypeptides of the invention consisting preferably of at least about 50, of at least about 100, of at least about 150, of at least about 200, of at least about 250, of at least about 300, of at least about 350, of at least about 400 to about 3000 proline and alanine amino acid residues and having random coil conformation show unexpectedly high values in relation to the hydrodynamic volume that would be estimated for a corresponding folded, globular protein based on the molecular weight. The following relates to biologically active, heterologous proteins or protein constructs comprising, inter alia, the biosynthetic random coil polypeptide (or segment thereof) as described and defined herein above which represent a prefered embodiment of the present invention. Without being bound by theory, it was surprisingly found in context of the present invention that the biosynthetic random coil polypeptide stretches as provided herein and consisting solely of proline and alanine can, even provide for a higher hydrodynamic volume than a corresponding biosynthetic random coil stretch having the same total number of amino acid residues but consisting solely of proline, alanine and serine (as provided in WO 2008/155134).

Common human plasma proteins such as serum albumin (HSA) and immunoglobulins (Igs), including humanized antibodies, show long half-lifes, typically of 2 to 3 weeks, which is attributable to their specific interaction with the neonatal Fc receptor (FcRn), leading to endosomal recycling (Ghetie (2002) Immunol Res, 25:97-113). In contrast, most other proteins of pharmaceutical interest, in particular recombinant antibody fragments, hormones, interferons, etc. suffer from rapid (blood) clearance. This is particularly true for proteins whose size is below the threshold value for kidney filtration of about 70 kDa (Caliceti (2003) Adv Drug Deliv Rev 55:1261-1277). In these cases the plasma half-life of an unmodified pharmaceutical protein may be considerably less than one hour, thus rendering it essentially useless for most therapeutic applications. In order to achieve sustained pharmacological action and also improved patient compliance—with required dosing intervals extending to days or even weeks—several strategies were previously established for purposes of biopharmaceutical drug development.

First, the recycling mechanism of natural plasma proteins has been employed by producing fusion proteins with the Fc portion of Igs, for example Enbrel®, a hybrid between the extracellular domain of TNFα receptor and human IgG1 (Goldenberg (1999) Clin Ther 21:75-87) or with serum albumin, for example ALBUFERON® (albinterferon alfa-2b, ZALBIN™, JOULFERON®), a corresponding fusion of IFNalpha with HSA (Osborn (2002) J Pharmacol Exp Ther 303:540-548). Albumin with its high plasma concentration of 600 μM has also been utilized in an indirect manner, serving as carrier vehicle for biopharmaceuticals that are equipped with an albumin-binding function, for example via fusion with a bacterial albumin-binding domain (ABD) from Streptococcal protein G (Makrides (1996) J Pharmacol Exp Ther 277:534-542) or with a peptide selected against HSA from a phage display library (Dennis (2002) J Biol Chem, 277:35035-35043; Nguyen (2006) Protein Eng Des Sel 19:291-297).

Second, a fundamentally different methodology for prolonging the plasma half-life of biopharmaceuticals is the conjugation with highly solvated and physiologically inert chemical polymers, thus effectively enlarging the hydrodynamic radius of the therapeutic protein beyond the glomerular pore size of approximately 3-5 nm (Caliceti (2003) loc. cit.). Covalent coupling under biochemically mild conditions with activated derivatives of poly-ethylene glycol (PEG), either randomly via Lys side chains (Clark (1996) J Biol Chem 271:21969-21977) or by means of specifically introduced Cys residues (Rosendahl (2005) BioProcess International: 52-60) has been moderately successful and is currently being applied in several approved drugs. Corresponding advantages have been achieved especially in conjunction with small proteins possessing specific pharmacological activity, for example Pegasys®, a chemically PEGylated recombinant IFNa-2a (Harris (2003) Nat Rev Drug Discov, 2:214-221; Walsh (2003) Nat Biotechnol 21:865-870).

However, the chemical coupling of a biologically active protein with synthetic polymers has disadvantages with respect to biopharmaceutical development and production. Suitable PEG derivatives are expensive, especially as high purity is needed, and their conjugation with a recombinant protein requires additional in vitro processing and purification steps, which lower the yield and raise the manufacturing costs. In fact, PEG is often contaminated with aldehydes and peroxides (Ray (1985) Anal Biochem 146:307-312) and it is intrinsically prone to chemical degradation upon storage in the presence of oxygen. Also, the pharmaceutical function of a therapeutic protein may be hampered if amino acid side chains in the vicinity of its biochemical active site become modified by the PEGylation process. Furthermore, chemical coupling with synthetic polymers usually results in a heterogeneous mixture of molecules which may show a substantial variance of in vivo activity.

Third, the use of glycosylation analogs of biologically active proteins in which new N-linked glycosylation consensus sequences are introduced has been proposed to prolong plasma half-life; see WO 02/02597; Perlman (2003) J Clin Endocrinol Metab 88:2327-2335; or Elliott (2003) Nat Biotechnol 21:414-420). The described glycoengineered proteins, however, displayed an altered in vivo activity, which indicates that the new carbohydrate side chains influence the biological activity of the engineered protein. Moreover, the additional carbohydrate side chains are likely to increase the antigenicity of the resulting biological active molecules, which raises substantial safety concerns. Furthermore, fusion proteins comprising the Trypanosoma cruzi derived artificial repetitive sequence PSTAD have been reported to induce a prolonged plasma half-life of trans-sialidase (Alvarez (2004) JBC 279:3375-3381). Yet, such Trypanosoma cruzi derived repeats have been reported to induce a humoral immune response (Alvarez (2004) loc. cit.). Accordingly, alternative strategies to prolong the action of biologically active proteins are desired.

The biosynthetic amino acid sequences/polypeptides as disclosed herein and consisting solely of proline and alanine according to the invention were surprisingly found to adopt random coil conformation in particular under physiological conditions. Therefore, they are advantageous molecules to provide for the herein below defined “second domain” of the biologically active protein(s)/polypeptide(s), i.e. comprising a polypeptide stretch that forms under physiological conditions a random coil conformation and thereby mediates an increased in vivo and/or in vitro stability to biologically active (“functional”) protein(s) or polypeptide(s), in particular, an increased plasma half-life. The hydrodynamic volume of a functional protein that is fused to said random coil domain is dramatically increased as can be estimated by using standard methods mentioned herein. Since the random coil domain is thought not to interfere with the biological activity of the first domain of the biologically active protein, the biological activity mediated by the functional protein of interest to which it is fused is essentially preserved. Moreover, the amino acid polymers/polypeptides that form random coil domain as disclosed herein are thought to be biologically largely inert, especially with respect to proteolysis in blood plasma, immunogenicity, isoelectric point/electrostatic behaviour, binding to cell surface receptors as well as internalisation, but still biodegradable, which provides clear advantages over synthetic polymers such as PEG.

In accordance with the above, the present invention relates to a biologically active protein comprising the herein described biosynthetic random coil polypeptide. Such a biologically active protein/protein construct comprising the biosynthetic random coil polypeptide described herein is a heterologous biological active protein/protein construct. In particular, herein disclosed is/are also (a) biologically active, heterologous protein(s) comprising or consisting of at least two domains wherein

-   (a) a first domain of said at least two domains comprises or     consists of an amino acid sequence having and/or mediating said     biological activity; and -   (b) a second domain of said at least two domains comprises or     consists of the herein described and defined random coil polypeptide     or polypeptide segment.

It is of note that in accordance with the present invention that “first domain” and said “second domain” relate to protein stretches that are not naturally occurring within the same protein or that are not expected to be part of the same hypothetical protein as encoded by a coding nucleic acid sequence (like an open reading frame) as found in nature.

The definitions and explanations given herein above in context of the random coil polypeptide or polypeptide segment thereof apply, mutatis mutandis, in the context of biologically active proteins comprising said random coil polypeptide (or (a) polypeptide segment(s) thereof).

Preferably, said random coil conformation mediates an increased in vivo and/or in vitro stability of said biologically active protein, like the in vivo and/or in vitro stability in biological samples or in physiological environments.

For example, it is envisaged herein that proteins comprising a herein defined, additional “second domain” adopting a random coil conformation in aqueous solution or under physiological conditions (for example polymers consisting of about 200 or about 400 or about 600 amino acid residues and comprising PA #1/SEQ ID NO. 1, PA #2/SEQ ID NO. 2, PA #3/SEQ ID NO. 3, PA #4/SEQ ID NO. 4, PA #5/SEQ ID NO. 5, PA #6/SEQ ID NO. 6 and/or P1A1/SEQ ID NO. 51 as “building blocks”) have an advantageous serum stability or plasma half-life, even in vivo, (in particular if intravenously administered) as compared to a control lacking said random coil conformation.

In WO 2008/155134 (as discussed herein above) it has been shown that biologically active proteins which comprise a domain with an amino acid sequence adopting a random coil conformation have an increased in vivo and/or in vitro stability. The random coil domains disclosed in WO 2008/155134 consist, in particular, of proline, alanine, and serine (PAS) residues. The presence of these three residues is described in this prior art document as an essential requirement for the formation of a stable and soluble random coil in aqueous solution.

As discussed in the introduction herein above, WO 2007/103515 describes unstructured recombinant polymers which comprise as main constituents a large variety of amino acids, inter alia, glycine, aspartate, alanine, serine, threonine, glutamate and proline. However, the term “unstructured recombinant polymer” has, in contrast to the terms “biosynthetic” and “random coil”, no recognized, clear meaning.

Also mentioned herein above was WO 2006/081249. This document describes protein conjugates comprising a biologically active protein coupled to a polypeptide comprising 2 to 500 units of an amino acid repeat having Gly, Asn, and Gln as a major constituent and Ser, Thr, Asp, Gln, Glu, His, and Asn as a minor constituent. Said protein conjugates are described to have either an increased or a decreased plasma half-life when compared to the unconjugated biologically active protein. WO 2006/081249, however, does not provide any teaching to predict whether a specific amino acid repeat reduces or augments the plasma half-life of the conjugate. Moreover, WO 2006/081249 does not teach or suggest that the plasma half-life of proteins can be increased when the conjugated protein comprises an amino acid repeat that forms random coil conformation as shown in the present invention. Furthermore, the amino acid repeats disclosed in WO 2006/081249 comprise at least two residues selected from Gly, Asn, and Gln, which is in clear contrast with the biosynthetic random coil polypeptides of the present invention which comprise an amino acid sequence that solely consists of proline and alanine amino acid residues.

Surprisingly, it has been found herein that biosynthetic random coil amino acid sequences as provided herein which, in contrast to the prior art, solely comprise proline and alanine residues (i.e. which preferably do not comprise a substantial amount of any other amino acid, also not a substantial amount of serine or no serine at all) do also form a useful random coil structure. This is particularly unexpected given the disclosure in WO 2008/155134 of fusion proteins with a domain composed only of serine and alanine (SA) residues, i.e. where proline residues were omitted, demonstrating that such a domain comprising only two types of amino acids did not form a random coil, but a β-sheet structure. These serine-alanine domains did also not show such an increased hydrodynamic volume as observed with “PAS” or, in particular, with the “P/A” sequences as provided herein.

As used herein, the term “biological activity” describes the biological effect of a substance on living matter. Accordingly, the terms “biologically active protein” as used herein relate to proteins that are capable of inducing a biological effect in living cells/organisms that are exposed to said protein or polypeptide. Yet, it is of note that in the context of the present invention, the term “biologically active protein” relates to the whole protein of the invention which both comprises an amino acid sequence having and/or mediating said biological activity (said first domain) and the inventive amino acid sequence adopting/forming random coil conformation and consisting solely of proline and alanine (said second domain).

Accordingly, the terms “amino acid sequence having and/or mediating biological activity” or “amino acid sequence with biological activity” as used herein to the above-defined “first domain” of the biologically active protein of the invention, which mediates or has or is capable of mediating or having the above defined “biological activity”. Also comprised in the terms “amino acid sequence having and/or mediating biological activity” or “amino acid sequence with biological activity” are any proteins of interest (and functional fragments thereof, such as antibody fragments, fragments comprising extracellular or intracellular domain(s) of a membrane receptor, truncated forms of a growth factor or cytokine and the like), the half-life of which, either in vivo or in vitro, needs to be prolonged. In one embodiment of this invention, the amino acid sequence having and/or mediating biological activity in accordance with the present invention may be deduced from any “protein of interest”, i.e. any protein of pharmaceutical or biological interest or any protein that is useful as a therapeutic/diagnostic agent.

Accordingly, the biologically active proteins may comprise a first domain comprising a biologically active amino acid sequence which is derived from naturally produced polypeptides or polypeptides produced by recombinant DNA technology. In a preferred embodiment, the protein of interest may be selected from the group consisting of binding proteins/binding molecules, immunoglobulins, antibody fragments, transport proteins, membrane receptors, signaling proteins/peptides such as cytokines, growth factors, hormones or enzymes and the like.

As explained herein above, the random coil polypeptide (or polypeptide segment) comprised in the second domain of the biologically active protein forms the random coil conformation in particular under physiological conditions. This is particularly relevant in context of biologically active proteins which may form part of a pharmaceutical composition that is to be administered to a subject or patient.

It is of note that the inventive biosynthetic random coil domain (said “second domain”) of the biologically active protein natively (ie. under physiologic conditions) adopts/forms/has random coil conformation, in particular in vivo and when administered to mammals or human patients in need of medical intervention. In contrast, it is known in the art that proteins having a non-random secondary and/or tertiary structure as native conformation tend to adopt a random coil conformation under non-physiological conditions (i.e. under denaturing conditions). However, such denatured proteins have completely different characteristics compared to the biologically active protein comprising the random coil polypeptide of the present invention. Hence, it is the gist of this invention that the “biologically active protein” and the biologically active part of the fusion proteins/fusion constructs as provided herein maintain their biological function also when combined and/or linked with the biosynthetic random coil polypeptide (or polypeptide segment) of this invention.

Furthermore, the random coil polypeptide (or polypeptide segment) retains solubility under physiological conditions. Accordingly, it is also envisaged that the protein construct of the present invention (comprising the above defined “first” and “second domain”) may comprise the “second”, random coil forming/adopting domain transiently or temporarily not in random coil conformation, for example, when in form of a specific composition, like a lyophylisate or dried composition. Yet, it is important that such a “second domain” of the inventive protein construct again adopts after, e.g., reconstitution in corresponding buffers (preferably “physiological” buffers/excipients and/or solvents), the herein defined random coil conformation. Said “second domain” is (if necessary, after corresponding reconstitution) capable of mediating an increased in vivo and/or in vitro stability of the inventive biologically active protein. It is preferred herein that the “second domain” as defined herein consists of the random coil polypeptide (or polypeptide segment) of the present invention.

As used herein, the term “domain” relates to any region/part of an amino acid sequence that is capable of autonomously adopting a specific structure and/or function. In the context of the present invention, accordingly, a “domain” may represent a functional domain or a structural domain. As described herein, the proteins of the present invention comprise at least one domain/part having and/or mediating biological activity and at least one domain/part forming random coil conformation. Yet, the proteins of the invention also may consist of more than two domains and may comprise e.g. an additional linker or spacer structure between the herein defined two domains/parts or another domain/part like, e.g. a protease sensitive cleavage site, an affinity tag such as the His₆-tag or the Strep-tag, a signal peptide, retention peptide, a targeting peptide like a membrane translocation peptide or additional effector domains like antibody fragments for tumour targeting associated with an anti-tumour toxin or an enzyme for prodrug-activation etc.

In another embodiment, the biologically active protein of the invention has a hydrodynamic volume as determined by analytical gel filtration (also known as size exclusion chromatography, SEC) of at least 50 kDa, preferably of at least 70 kDa, more preferably of at least 80 kDa, even more preferably of at least 100 kDa, particularly preferably of at least 125 kDa and most preferably of at least 150 kDa. The person skilled in the art is readily capable of determining the hydrodynamic volume of specific proteins. Exemplary methods have been described herein above in context of the random coil polypeptide. A skilled person is easily in the position to adapt such methods also in context of the biologically active protein of the present invention. As described herein below, the hydrodynamic volume of the biologically active proteins of the invention that comprise the above defined second domain, i.e. the domain comprising or consisting of the herein provided random coil polypeptide (or segment thereof) are shown to have an unexpectedly large hydrodynamic volume in relation to the estimated hydrodynamic volume for a corresponding folded, globular protein based on their molecular weight or number/composition of amino acid residues.

It should be noted that the first domain comprising an “amino acid sequence having and/or mediating biological activity” may also adopt its biological activity in the context of or after association with another polypeptide or amino acid sequence. For example, the Fab fragment of an antibody such as the one of the anti-tumour antibody Herceptin (Eigenbrot (1993) J. Mol. Biol. 229:969-995) consists of two different polypeptide chain, the immunoglobulin light chain and a fragment of the immunoglobulin heavy chain, which may furthermore be linked via (an) interchain disulfide bond(s). According to the present invention, it may be sufficient to link one of those chains (e.g. via gene fusion) to the random coil polypeptide (or polypeptide segment) while the full biologically active protein is reconstituted by means of association with the other chain. Such reconstitution may be achieved, for example, by co-expression of the different polypeptides (on the one hand a fusion protein of one chain and the random coil polypeptide, on the other hand the other chain) in the same host cell, as described in the appended examples, or by reconstitution in vitro, for example, as part of a refolding protocol.

Accordingly, also such proteins (comprising tow separate polypeptide chains) are considered as biologically active proteins in accordance with the present invention. In such a case, the first domain as defined herein may comprise two separate polypeptide chains which are linked only non-covalently. Furthermore, the independent chains of the biologically active protein/domain may each be linked to the random coil polypeptide (or polypeptide segment). Beside antibody fragments there are many other homo- or hetero-oligomeric proteins of interest (for example, insulin, hemoglobin and the like) that are composed of several associated polypeptide chains and which are subject to this invention.

As used herein, the term “binding protein” relates to a molecule that is able to specifically interact with (a) potential binding partner(s) so that it is able to discriminate between said potential binding partner(s) and a plurality of different molecules as said potential binding partner(s) to such an extent that, from a pool of said plurality of different molecules as potential binding partner(s), only said potential binding partner(s) is/are bound, or is/are significantly bound. Methods for the measurement of binding between a binding protein and a potential binding partner are known in the art and can be routinely performed, e.g., by using ELISA, isothermal titration calorimetry, equilibrium dialysis, pull down assays, surface plasmon resonance or a Biacore apparatus. Exemplary binding proteins/binding molecules which are useful in the context of the present invention include, but are not limited to antibodies, antibody fragments such as Fab fragments, F(ab′)₂ fragments, single chain variable fragments (scFv), isolated variable regions of antibodies (VL and/or VH regions), CDRs, single domain antibodies/immunoglobulins, CDR-derived peptidomimetics, lectins, immunoglobulin domains, fibronectin domains, protein A domains, SH3 domains, ankyrin repeat domains, lipocalins or various types of scaffold-derived binding proteins as described, for example, in Skerra (2000) J Mol Recognit 13:167-187, Gebauer (2009) Curr Opin Chem Biol 13:245-255, Binz (2005) Nat Biotechnol 23:1257-1268 or Nelson (2009) Nat Biotechnol 27:331-337.

Other exemplary biologically active proteins of interest (in particular proteins comprised in the first domain or constituting/being the first domain of the biologically active protein) which are useful in the context of the present invention include, but are not limited to, granulocyte colony stimulating factor, human growth hormone, alpha-interferon, beta-interferon, gamma-interferon, lambda-interferone, tumor necrosis factor, erythropoietin, coagulation factors such as coagulation factor VIII, coagulation factor VIIa, coagulation factor IX, gp120/gp160, soluble tumor necrosis factor I and II receptor, thrombolytics such as reteplase, peptides with metabolic effects such as GLP-1 or exendin-4, immunosuppressive/immunoregulatory proteins like interleukin-1 receptor antagonists or anakinra, interleukin-2 and neutrophil gelatinase-associated lipocalin or other natural or engineered lipocalins or those proteins or compounds listed, for example, in Walsh (2003) Nat Biotechnol 21:865-870 or Walsh (2004) Eur J Pharm Biopharm 58:185-196 or listed in online databases such as biopharma.com/approvals.html or drugbank.ca. Further biologically active proteins (in particular proteins comprised in the first domain or constituting/being the first domain of the biologically active protein) which may be employed in context of the present invention are, inter alia, follicle-stimulating hormone, glucocerebrosidase, thymosin alpha 1, glucagon, somatostatin, adenosine deaminase, interleukin 11, hematide, leptin, interleukin-20, interleukin-22 receptor subunit alpha (IL-22ra), interleukin-22, hyaluronidase, fibroblast growth factor 18, fibroblast growth factor 21, glucagon-like peptide 1, osteoprotegerin, IL-18 binding protein, growth hormone releasing factor, soluble TACI receptor, thrombospondin-1, soluble VEGF receptor Flt-1, α-galactosidase A, myostatin antagonist, gastric inhibitory polypeptide, alpha-1 antitrypsin, IL-4 mutein, and the like. As will be evident from the disclosure herein, the present invention also relates to comprising the biosynthetic random coil proline/alanine polypeptide or proline/alanine polypeptide segment and pharmaceutically or medically useful molecules, like small molecules, peptides or biomacromolecules such as proteins, nucleic acids, carbohydrates, lipid vesicles and the like, in particular pharmaceutically or medically useful proteins, like (but not limited to) binding proteins/binding molecules, immunoglobulins, antibody fragments, transport proteins, membrane receptors, signaling proteins/peptides, cytokines, growth factors, hormones or enzymes and the like may be comprised in the herein defined drug constructs btu they may also be part of the herein defined biologically active, heterologous protein comprising or consisting of said defined at least two domains. In such a case, said particular pharmaceutically or medically useful proteins (or functional fragments thereof) may be the “first domain” of said at least two domains comprising or consisting of an amino acid sequence having and/or mediating said biological activity Functional fragments, in this context, are fragments of said pharmaceutically or medically useful proteins that are still capable to elucidate the desired biological or pharmaceutical response in vivo and/or in vitro and/or still have or mediate the desired biological activity.

The above-mentioned polypeptide linker/spacer, inserted between said first and said second domains, preferably comprises plural hydrophilic, peptide-bonded amino acids that are covalently linked to both domains. In yet another embodiment said polypeptide linker/spacer comprises a plasma protease cleavage site which allows the controlled release of said first domain comprising a polypeptide having and/or mediating a biological activity. Linkers of different types or lengths may be identified without undue burden to obtain optimal biological activity of specific proteins.

In a preferred embodiment, the biologically active proteins of the present invention are fusion proteins. A fusion protein as described herein may comprise at least one domain which can mediate a biological activity and at least one other domain which comprises the biosynthetic random coil polypeptide (or polypeptide segment) as described herein in a single multi-domain polypeptide. Again, it is of note that the present invention is not limited to fusion proteins wherein one domain mediates a biological activity. Also other “fusion proteins”/“fusion constructs” are provided herein wherein one part/domain is or comprises the inventive random coil polypeptide/polymer of proline/alanine and the other part/domain comprises another protein stretch/structure.

In particular, in the case of fusion proteins the random coil polypeptide (or polypeptide segment) according to this invention does not necessarily carry Pro or Ala residues at its amino or carboxyl terminus. In an alternative embodiment, the biologically active protein in accordance with the present invention may represent a protein conjugate wherein a protein of interest or a polypeptide/polypeptide stretch/peptide/amino acid sequence having and/or mediating biological activity is conjugated via a non-peptide bond to an amino acid sequence which forms/adopts random coil conformation, in particular, the random coil polypeptide (or polypeptide segment) as provided herein and consisting solely of proline and alanine residues. Non-peptide bonds that are useful for cross-linking proteins are known in the art with the biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues as provided herein. Such Non-peptide bonds may include disulfide bonds, e.g. between Cys side chains, thioether bonds or non-peptide covalent bonds induced by chemical cross-linkers, such as disuccinimidyl suberate (DSS) or sulfosuccinimidyl 4-[p-maleimidophenyl] butyrate (Sulfo-SMPB), metal-chelating/complexing groups, as well as non-covalent protein-protein interactions.

It is of note that the “biologically active protein” of the present invention may also comprise more than one “amino acid sequence having and/or mediating a biological activity”. Furthermore, the biologically active protein may also comprise more than biosynthetic random coil polypeptide (or segment thereof). In the simplest case, the biologically active protein consists of two domains, i.e. a first domain comprising an amino acid sequence having and/or mediating a biological activity and a second domain comprising the biosynthetic polypeptide (or segment thereof). It is of note that the present invention is not limited to “biologically or therapeutically active proteins” linked to the herein disclosed biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues. Also other proteins or molecules of interest, as relevant for other industries, like food or beverage industry, cosmetic industry and the like, may be manufactured by the means and methods provided herein.

The person skilled in the art is aware that the “domain comprising an amino acid sequence having and/or mediating a biological activity” and the “second domain comprising the random coil polypeptide (or segment thereof) as comprised in the biologically active proteins of the invention may be organized in a specific order.

Accordingly, and in the context of the invention, the order of the herein defined “first” and “second” domain of the inventive biologically active polypeptide may be arranged in an order, whereby said “first domain” (i.e. protein of interest; “amino acid sequence having and/or mediating said biological activity”) is located at the amino (N-) terminus and said “second domain” (i.e. the domain that comprises the herein provided random coil polypeptide (or segment thereof)) is located at the carboxy (C-) terminus of the biologically active protein. However, this order may also be reversed, e.g. said “first domain” (i.e. protein of interest; “amino acid sequence having and/or mediating said biological activity”) is located at the carboxy (C-) terminus and said “second domain” (i.e. the domain that comprises the herein provided random coil polypeptide (or segment thereof)) is located at the amino (N-) terminus of the biologically active protein. If the biologically active protein consists only of one first domain and one second domain, the domain order may, accordingly, be (from N-terminus to C-terminus): first domain (amino acid sequence having and/or mediating a biological activity)-second domain (random coil polypeptide (or segment thereof)). Vice versa, the domain order may be (from N-terminus to C-terminus): second domain (random coil polypeptide (or segment thereof))-first domain (amino acid sequence having and/or mediating a biological activity).

It is also envisaged that more than one domain comprising or consisting of an amino acid sequence having and/or mediating said biological activity are to be used in context of the inventive protein construct. For example, the biologically active protein may comprise two “first domain”, i.e. two specific amino acid sequences having and/or mediating a biological activity, whereby this biological activity may be the same or a different activity. If the biologically active protein consists of two such “first domains”, i.e two specific amino acid sequences having and/or mediating a biological activity, and one “second domain” (comprising the biosynthetic random coil polypeptide (or segment thereof), the domain order may be (from N-terminus to C-terminus): first domain (amino acid sequence having and/or mediating a specific biological activity)-second domain (random coil polypeptide (or segment thereof))-first domain (amino acid sequence having and/or mediating a specific (optionally different) biological activity).

The same explanations apply in cases where the biologically active protein comprises more than one “second domain” (i.e. the biologically active protein comprises more than one random coil polypeptide (or segment thereof). If the biologically active protein consists of two such “second domains”, i.e two domains comprising the biosynthetic random coil polypeptide (or segment thereof), and one “first domain” (comprising an amino acid sequence having and/or mediating a biological activity), the domain order may be (from N-terminus to C-terminus): second domain (random coil polypeptide (or segment thereof))-first domain (amino acid sequence having and/or mediating a specific biological activity)-second domain (random coil polypeptide (or segment thereof)). If the biologically active protein comprises more than one “second domain” it is envisaged herein that these “second domains” may be identical or may be different.

As mentioned above, the biologically active protein may comprise more than one “first domain”, i.e. more than one specific amino acid sequences having and/or mediating a biological activity and more than one “second domain” (biosynthetic random coil polypeptide (or segment thereof)) whereby these “first domains” may be identical or different and/or whereby said “second domains” may be identical or different. In such cases the following, exemplary domain orders are conceivable (from N-terminus to C-terminus):

-   -   first domain (amino acid sequence having and/or mediating a         specific biological activity)-second domain (random coil         polypeptide (or segment thereof))-first domain (amino acid         sequence having and/or mediating a specific biological         activity)-second domain (random coil polypeptide (or segment         thereof));     -   second domain (random coil polypeptide (or segment         thereof))-first domain (amino acid sequence having and/or         mediating a specific biological activity)-first domain (amino         acid sequence having and/or mediating a specific biological         activity)-second domain (random coil polypeptide (or segment         thereof));     -   first domain (amino acid sequence having and/or mediating a         specific biological activity)-second domain (random coil         polypeptide (or segment thereof))-second domain (random coil         polypeptide (or segment thereof))-first domain (amino acid         sequence having and/or mediating a specific biological         activity);     -   second domain (random coil polypeptide (or segment         thereof))-first domain (amino acid sequence having and/or         mediating a specific biological activity)-second domain (random         coil polypeptide (or segment thereof))-first domain (amino acid         sequence having and/or mediating a specific biological         activity);     -   second domain (random coil polypeptide (or segment         thereof))-second domain (random coil polypeptide (or segment         thereof))-first domain (amino acid sequence having and/or         mediating a specific biological activity)-first domain (amino         acid sequence having and/or mediating a specific biological         activity); or     -   first domain (amino acid sequence having and/or mediating a         specific biological activity)-first domain (amino acid sequence         having and/or mediating a specific biological activity)-second         domain (random coil polypeptide (or segment thereof))-second         domain (random coil polypeptide (or segment thereof)).

For a person skilled in the art further corresponding domain orders (in particular in cases where more than two “first domains” or “more than two “second domains” are comprised in the biologically active protein) are easily conceivable.

As with all embodiments of the present inventive polypeptide/biologically active protein, said domain(s) comprising an amino acid sequence having and/or mediating the said biological activity may also be a biologically active fragment of a given protein with a desired biological function. Therefore, the herein defined “second domain” (preferably comprising the herein provided random coil polypeptide (or segment thereof)) may also be located between two biologically active fragments of a protein of interest or between biologically active fragments of two proteins of interest. All the explanations and definitions given herein above in context of “full length” proteins/polypeptides of interest (i.e. when the amino acid sequences has/mediates a certain biological activity on its own) apply, mutatis mutandis, in context of such fragments.

Again the above invention is not limited to the constructs that comprise a “domain” with a “biological active function”. The constructs of the present invention may also comprise domains with other functions and are not limited to biological activities. These are merely embodiments of the present invention and it is evident for the skilled artisan that other constructs can easily be made and used without deferring from the gist of the present invention. Accordingly, the herein said in context of “amino acid sequence having and/or mediating a specific biological activity” applies, mutatis mutandis, for other constructs, for example constructs to be used in other technical fields, like in cosmetics, food processing, dairy products, paper production, etc. As mentioned herein above, the biosynthetic polypeptides/polymers of the present invention can also be used to be linked with e.g. small molecules and the like.

Again, it has to be pointed out that the term “amino acid sequence having and/or mediating first biological activity” is not limited to full-length polypeptides that have and/or mediate said biological activity or function, but also to biologically and/or pharmacologically active fragments thereof. Especially, but not only, in a context wherein two or more “first domains” as defined herein are comprised in the inventive “biologically active protein” it is also envisaged that these “first domains” are or represent different parts of a protein complex or fragments of such parts of protein complex.

As exemplified herein below, the biologically active proteins of the invention which are modified to comprise a random coil polypeptide surprisingly exhibit an increased in vivo and/or in vitro stability when compared to unmodified biologically active proteins that lack said random coil domain. As used herein, the term “in vivo stability” relates to the capacity of a specific substance that is administered to the living body to remain biologically available and biologically active. In vivo, a substance may be removed and/or inactivated due to excretion, kidney filtration, liver uptake, aggregation, degradation and/or other metabolic processes. Accordingly, in the context of the present invention biologically active proteins that have an increased in vivo stability may be less rapidly excreted through the kidneys (urine) or via the feces and/or may be more stable against proteolysis, in particular against in vivo proteolysis in biological fluids, like blood, liquor cerebrospinalis, peritoneal fluid, and lymph. In one embodiment, the increased in vivo stability of a biologically active protein manifests in a prolonged plasma half-life of said biologically active protein. In particular, the increased in vivo stability of the biologically active protein is a prolonged plasma half-life of said biologically active protein comprising said second domain when compared to the biologically active protein lacking the second domain.

Methods for measuring the in vivo stability of biologically active proteins are known in the art. As exemplified herein below, biologically active proteins may be specifically detected in the blood plasma using Western blotting techniques or enzyme linked immunosorbent assay (ELISA). Yet, the person skilled in the art is aware that other methods may be employed to specifically measure the plasma half-life of a protein of interest. Such methods include, but are not limited to the physical detection of a radioactively labelled protein of interest. Methods for radioactive labelling of proteins e.g. by radioiodination are known in the art.

The term “increased in vitro stability” as used herein relates to the capacity of a biologically active protein to resist degradation and/or aggregation and to maintain its original biological activity in an in vitro environment. Methods for measuring the biological activity of biologically active proteins are well known in the art.

Furthermore, a drug conjugate is provided which comprises the herein described and defined random coil polypeptide or polypeptide segment and a small molecule drug that is conjugated to said random coil polypeptide or polypeptide segment. Non-limiting examples of the small molecules are digoxigenin, fluorescein doxorubicin, calicheamicin, camptothecin, fumagillin, dexamethasone, geldanamycin, paclitaxel, docetaxel, irinotecan, cyclosporine, buprenorphine, naltrexone, naloxone, vindesine, vancomycin, risperidone, aripiprazole, palonosetron, granisetron, cytarabine, NX1838, leuprolide, goserelin, buserelin, octreotide, teduglutide, cilengitide, abarelix, enfuvirtide, ghrelin and derivatives, tubulysins, platin derivatives, alpha 4 integrin inhibitors, antisense nucleic acids, small interference RNAs, micro RNAs, steroids, DNA or RNA aptamers, peptides, peptidomimetics. In general, the present invention also relates to drug constructs comprising the herein defined random coil polypeptide or polypeptide segment and in particular pharmaceutically or medically useful molecules, like small molecules, peptides or biomacromolecules such as proteins, nucleic acids, carbohydrates, lipid vesicles and the like. In the appended illustrative experimental part (see, e.g. Example 22) the successful generation of constructs/conjugates of the present invention are provided, also constructs wherein “small chemical molecules” have been conjugated to the herein disclosed random coil polypeptide. Therefore, the present Figures and experimental information in the corresponding figure legends provide for illustrative examples, wherein the herein disclosed drug conjugates comprise (i) a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, and (ii) a small molecule, which is, as illustration, selected from digoxigenin and fluorescein. It is of note that these are not only academic examples. Fluorescein or fluorescein derivates are are commonly used as diagnostics, and medical fluorescein solutions are sold under the trade names Fluoescite®, AK-FLUOR® or Fluress®. Such compounds can certainly profit from the means and methods provided herein. Digoxigenin forms the steroid part of digoxin, a well known secondary plant metabolite with cardioactive function which furthermore contains three digitoxose sugars. Digoxin, and to a lesser extent the closely related compound digitoxin, are widely used for the treatment of ventricular tachyarrhythmias and congestive heart failure (Hauptman (1999) Circulation 99: 1265-1270). All cardioactive steroids are potent and highly specific inhibitors of the Na⁺/K⁺-ATPase located in the cellular plasma membrane, thereby exerting sympatholytic or positive inotropic effects.

The definitions and explanations given herein above in context of the random coil polypeptide or polypeptide segment thereof apply, mutatis mutandis, in context of drug conjugate comprising the random coil polypeptide (or polypeptide segment thereof) and a drug selected from the group consisting of (a) a biologically active protein or a polypeptide that comprises or that is an amino acid sequence that has or mediates a biological activity and (b) a small molecule drug.

The amino acid polymer forming random coil conformation/the random coil polypeptide (or segment thereof) as defined and provided herein can be conjugated to a small molecule/small molecule drug. By this means, plasma half-life and/or solubility of the small molecule/small molecule drug may be increased, unspecific toxicity may be decreased, and the prolonged exposure of active drug to target cells or structures in the body may result in enhanced pharmacodynamics.

A site-specific conjugation of the N-terminus of the random coil polypeptide with an activated drug derivative, e.g. as N-hydroxysuccinimide (NHS) ester derivative (Hermanson (1996) Bioconjugate Techniques, Academic Press, San Diego, Calif.), is possible. Generally, the N-terminal amino group can be chemically coupled with a wide variety of functional groups such as aldehydes and ketones (to form Schiff bases, which may be reduced to amines using sodium borohydride or sodium cyanoborohydride, for example) or to activated carbonic acid derivatives (anhydrides, chlorides, esters and the like, to form amides) or to other reactive chemicals such as isocyanates, isothiocyanates, sulfonyl chlorides etc. Also, the N-terminus of the amino acid polymer/polypeptide can first be modified with a suitable protective group, for example an acetyl group, a BOC group or an FMOC group (Jakubke (1996) Peptide. Spektrum Akdemischer Verlag, Heidelberg, Germany). Furthermore, the amino terminus may be protected by a pyroglutamyl group, which can form from an encoded Gln amino acid residue preceding the Pro/Ala polypeptide or polypeptide segment. After activation of the C-terminal carboxylate group, e.g. using the common reagents EDC (N-(3-dimethylaminopropyl)-N′-ethylcarbodiimide) and NHS, site-specific coupling to the C-terminus of the protected random coil polypeptide can be achieved if the drug carries a free amino group, for example.

Alternatively, the N-terminus or the C-terminus of the amino acid polymer forming random coil conformation/the random coil polypeptide can be modified with a commercially available linker reagent providing a maleimide group, thus allowing chemical coupling to a thiol group as part of the drug molecule. In this manner uniform drug conjugates can be easily obtained. Similar techniques, which are well known in the art (Hermanson (1996) loc. cit.), can be used to couple the random coil polypeptide to a peptide or even to a protein drug. Such peptides or proteins can easily be prepared carrying a Lys or Cys side chain, which allows their in vitro coupling to the amino acid polymer forming random coil conformation via NHS ester or maleimide active groups. Generally, similar drug conjugates can be prepared with fusion proteins comprising the random coil polypeptide (or segment thereof). Yet, and as illustrated in the appended Examples and Figures the present invention also provides for the preparation of a random coil polypeptides or a random coil polypeptide segments as comprised in the innovative conjugates of the present invention.

As an alternative to a single site-specific conjugation the random coil polypeptide may be equipped with additional side chains, at the N- or C-terminus or internally, suitable for chemical modification such as lysine residues with their ε-amino groups, cysteine residues with their thiol groups, or even non-natural amino acids, allowing the conjugation of multiple small molecules using, for example, NHS ester or maleimide active groups.

Apart from stable conjugation, a prodrug may be linked transiently to the random coil polypeptide. The linkage can be designed to be cleaved in vivo, in a predictable fashion, either via an enzymatic mechanism or by slow hydrolysis initiated at physiological pH similarly as, for example, the poorly soluble antitumor agent camptothecin was conjugated to a PEG polymer, thus achieving increased biodistribution, decreased toxicity, enhanced efficacy and tumor accumulation (Conover (1998) Cancer Chemother Pharmacol, 42:407-414). Examples for further prodrugs are chemotherapeutic agents like docetaxel (Liu (2008) J Pharm Sci. 97:3274-3290), doxorubicin (Veronese (2005) Bioconjugate Chem. 16: 775-784) or paclitaxel (Greenwald (2001) J Control Release 74:159-171).

Furthermore, the small molecule may be coupled to a fusion protein comprising the amino acid polymer/polypeptide genetically fused to a targeting domain, e.g. an antibody fragment, thus resulting in a specific delivery of the small molecule drug. In the latter case immunotoxins can be easily generated by conjugation with a cytotoxic small molecule if the targeting domain is directed against a cell-surface receptor which undergoes internalization, for example.

In accordance with the above, the present invention also relates, therefore, to the provision of the herein disclosed biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues for further and additional coupling with other compounds of choice. Said further and/or additional coupling may be and/or may comprise the first coupling of said biosynthetic random coil polypeptide or biosynthetic random coil polypeptide segment with or to another compound.

In another embodiment, the present invention relates to nucleic acid molecules encoding the random coil polypeptides (or segments thereof) or biologically active proteins as described herein. Accordingly, said nucleic acid molecule may comprise a nucleic acid sequence encoding a polypeptide having biological activity and a nucleic acid sequence encoding the random coil polypeptide (or segment thereof) . . . . The term “nucleic acid molecule”, as used herein, is intended to include nucleic acid molecules such as DNA molecules and RNA molecules. Said nucleic acid molecule may be single-stranded or double-stranded, but preferably is double-stranded DNA. Preferably, said nucleic acid molecule may be comprised in a vector.

Accordingly, the present invention also relates to a nucleic acid molecule encoding the random coil polypeptide or polypeptide segment as comprised in the conjugates provided herein, like a drug conjugate as defined herein, or a nucleic acid molecule encoding a protein conjugate that comprises a biologically active protein as defined above and that comprises, additionally, a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues.

In one embodiment a nucleic acid molecule is provided that encodes a conjugate, like a drug conjugate or food conjugate as defined above, said nucleic acid molecule comprising

-   (i) a nucleic acid sequence encoding a translated amino acid and/or     a leader sequence; -   (ii) a nucleic acid sequence encoding a biosynthetic random coil     polypeptide or polypeptide segment comprising an amino acid sequence     consisting solely of proline and alanine amino acid residues,     wherein said amino acid sequence consists of at least 50 proline     (Pro) and alanine (Ala) amino acid residues; -   (iii) a nucleic acid sequence encoding biologically active protein     or said a polypeptide that comprises or that is an amino acid     sequence that has or that mediates a biological activity or a     protein of interest, like a protein to be employed in other     industrial areas like the food industry; and -   (iv) a nucleic acid sequence that represents or is a translational     stop codon.

The above mentioned “translated amino acid and/or a leader sequence” under (i) may for example be the starting “M”, i.e. a methionine derived from a corresponding starting codon, it may also comprise non-translated sequences of an mRNA like the 5′ sequence up to a start codon which comprises for example a ribosome binding site. Such a sequence may however also comprise classical leader and/or signal sequences for example for secretion of an expressed protein into the periplasm or in a culture medium. Prokaryotic signal peptides are for example OmpA, MalE, PhoA, DsbA, pelB, Afa, npr, STII. Eukaryotic signal peptides are for example Honeybee melittin signal sequence, acidic glycoprotein gp67 signal sequence, mouse IgM signal sequence, hGH signal sequence.

Biologically active proteins or polypeptides that comprises or that is an amino acid sequence that has or that mediates a biological activity as well as other proteins of interest, like a protein to be employed in other industrial areas, have been provided herein above. Said embodiments apply, mutatis mutandis, for the nucleic acid molecule (part/segments (iii)) as illustrated herein above.

Translational stop codons to be employed in the nucleic acid molecule provided herein are well known in the art and are, e.g. codons UAA, UAG or UGA.

In one embodiment of the nucleic acid molecule as provided herein above said nucleic acid molecule parts/segments (ii) and (iii) are interchanged in their position on said nucleic acid molecule encoding for a conjugate, like a drug conjugate or a food conjugate. Such a nucleic acid molecule would comprise the following order of parts/segments:

-   (i) a nucleic acid sequence encoding a translated amino acid and/or     a leader sequence; -   (ii) a nucleic acid sequence encoding biologically active protein or     said a polypeptide that comprises or that is an amino acid sequence     that has or that mediates a biological activity or a protein of     interest, like a protein to be employed in other industrial areas,     like the food industry; -   (iii) a nucleic acid sequence encoding a biosynthetic random coil     polypeptide or polypeptide segment comprising an amino acid sequence     consisting solely of proline and alanine amino acid residues,     wherein said amino acid sequence consists of at least 50 proline     (Pro) and alanine (Ala) amino acid residues; and -   (iv) a nucleic acid sequence that represents or is a translational     stop codon.

The nucleic acid molecules as provided herein above may also, optionally, comprise, between parts/segments (i) and (ii) and/or between parts/segments (ii) and (iii), a protease and/or a chemical cleavage site and/or a recognition site. Such chemical cleavage sites are well known in the art, and comprise for example specific, individual amino acid sequences (see, e.g. Lottspeich and Engels (Hrsg.) (2006) Bioanalytik. 2. Auflage. Spektrum Akademischer Verlag, Elsevier, München, Germany). For example, cyanogen bromide or cyanogen chloride cleaves the peptide bond following a Met residue; hydroxylamine cleaves the asparaginyl-glycyl bond; formic acid cleaves Asp-Pro; 2-(2′-nitrophenylsulfenyl)-3-methyl-3-bromoinolenine, 2-iodosobenzoic acid or N-chlorosuccinimide after Trp; 2-nitro-5-thiocyanatobenzoic acid after Cys. It is also envisaged and possible that the residue preceding the Pro/Ala polypeptide or polypeptide segment may be substituted to Met via site-directed mutagenesis and the resulting fusion protein can then be cleaved by BrCN. Similarly, other amino acid sequences comprising cleavage site can be introduced into the recombinant fusion protein or its encoding nucleic acid by way of site-directed mutagenesis.

Also useful protease recognition/cleavage sites are known in the art. These comprise, but are not limited to: trypsin, chymotrypsin, enterokinase, Tobacco Etch Virus (TEV) protease, PreScission protease, HRV 3C Protease, SUMO Protease, Sortase A, granzyme B, furin, thrombin, factor Xa or self cleavable inteins. Factor Xa hydrolyses the peptide bond at the C-terminal end of the amino acid sequence IleGluGlyArg, which may be inserted between the N-terminal fusion partner and the Pro/Ala polypeptide or polypeptide segment. A particularly simple method to achieve proteolytic cleavage would be by insertion or substitution of a Lys or Arg side chain at the N-terminal end of the Pro/Ala polypeptide or polypeptide segment followed by digest with trypsin, which does not cleave within the Pro/Ala polypeptide or polypeptide segment as long as internal Lys or Arg side chains are avoided. Illustrative recognition sites are, without being limited, D-D-D-D-K (enterokinase), ENLYFQ(G/S) (TEV protease), I-(E/D)-G-R (Factor Xa), L-E-V-L-F-Q-G-P (HRV 3C), R-X-(K/R)-R (Furin), LPXTG (Sortase A), L-V-P-R-G (Thrombin) or I-E-X-D-X-G (Granzyme B).

As is evident form the disclosure herein above, the present invention provides for recombinantly produced biosynthetic random coil polypeptides and polypeptide segments that can be conjugated with molecules of choice, like useful proteins, pharmaceutically active polypeptides or small molecules, diagnostically useful polypeptides or small molecules or, inter alia, other useful proteins or small molecules of other industrial areas, like food or paper industry or in oil recovery. Therefore, the present invention also provide for a nucleic acid encoding for a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, said nucleic acid molecule comprising

-   (i) a nucleic acid sequence encoding for a translated amino acid     and/or leader sequence; -   (ii) a nucleic acid sequence encoding for said a biosynthetic random     coil polypeptide or polypeptide segment comprising an amino acid     sequence consisting solely of proline and alanine amino acid     residues; and -   (iii) a nucleic acid sequence that represents or is a translational     stop codon.

Such a nucleic acid molecule may, optionally, comprise, between (i) and (ii) a protease and/or a chemical cleavage site and/or a recognition site).

Also for this nucleic acid molecule, the embodiments provided herein above in context of the first two described nucleic acid molecules (i.e. a protease and/or a chemical cleavage site and/or a recognition), apply here mutatis mutandis.

Useful and illustrative signal sequences to be employed in context of this invention comprise, but are not limited, prokaryotic sequences like: OmpA, MalE, PhoA, DsbA, pelB, Afa, npr, STII or eukaryotic sequences like: Honeybee melittin signal sequence, acidic glycoprotein gp67 signal sequence, mouse IgM signal sequence, hGH signal sequence

In particular the nucleic acid molecule encoding the biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues of the present invention is useful in methods as also provided herein below and as illustrated in the appended examples and figures. Such an expressed random coil polypeptide or random coil polypeptide segment can be isolated form, e.g. host cells expressing such a random coil polypeptide or random coil polypeptide segment. Such host cells may be transfected cells, for example with an vector as provided herein.

Therefore, it is envisaged to transfect cells with the nucleic acid molecule or vectors as described herein. In a further embodiment, the present invention relates to nucleic acid molecules which upon expression encode the random coil polypeptide (or segment thereof) or biologically active proteins of the invention. Yet, in a further embodiment, the present invention relates to nucleic acid molecules which upon expression encode the herein disclosed polypeptides that, entirely or in part, form/adopt random coil conformation in aqueous solution or under physiological conditions. Said nucleic acid molecules may be fused to suitable expression control sequences known in the art to ensure proper transcription and translation of the polypeptide as well as signal sequences to ensure cellular secretion or targeting to organelles. Such vectors may comprise further genes such as marker genes which allow for the selection of said vector in a suitable host cell and under suitable conditions.

Preferably, the nucleic acid molecule of the invention is comprised in a recombinant vector in which a nucleic acid molecule encoding the herein described biologically active protein is operatively linked to expression control sequences allowing expression in prokaryotic or eukaryotic cells. Expression of said nucleic acid molecule comprises transcription of the nucleic acid molecule into a translatable mRNA. Regulatory elements permitting expression in prokaryotic host cells comprise, e.g., the lambda PL, lac, trp, tac, ara, phoA, tet or T7 promoters in E. coli. Possible regulatory elements ensuring expression in eukaryotic cells, preferably mammalian cells or yeast, are well known to those skilled in the art. They usually comprise regulatory sequences ensuring initiation of transcription and optionally poly-A signals effecting termination of transcription and stabilization of the transcript. Additional regulatory elements may include transcriptional as well as translational enhancers, and/or naturally associated or heterologous promoter regions. Examples for regulatory elements permitting expression in eukaryotic host cells are the AOX1 or GAL1 promoters in yeast or the CMV, SV40, RSV (Rous sarcoma virus) promoters, CMV enhancer, SV40 enhancer or a globin intron in mammalian and other animal cells. Apart from elements which are responsible for the initiation of transcription such regulatory elements may also comprise transcription termination signals, such as the SV40-poly-A site or the tk-poly-A site, downstream of the coding region.

Methods which are well known to those skilled in the art can be used to construct recombinant vectors (see, for example, the techniques described in Sambrook (1989), Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory NY and Ausubel (1989), Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, NY). In this context, suitable expression vectors are known in the art such as Okayama-Berg cDNA expression vector pcDV1 (Pharmacia), pCDM8, pRc/CMV, pcDNA1, pcDNA3, pPICZalpha A (Invitrogen), or pSPORT1 (GIBCO BRL). Furthermore, depending on the expression system that is used, leader sequences capable of directing the polypeptide to a cellular compartment or secreting it into the culture medium may be added to the coding sequence of the nucleic acid molecule of the invention.

The present invention also relates to vectors, particularly plasmids, cosmids, viruses, and bacteriophages that are conventionally employed in genetic engineering, comprising a nucleic acid molecule encoding the the random coil polypeptide (or segment thereof) or the biologically active protein of the invention. Preferably, said vector is an expression vector and/or a gene transfer or targeting vector. Expression vectors derived from viruses such as retroviruses, vaccinia virus, adeno-associated virus, herpes viruses or bovine papilloma virus may be used for delivery of the polynucleotides or vector of the invention into targeted cell populations.

The vectors containing the nucleic acid molecules of the invention can be transfected into the host cell by well known methods, which vary depending on the type of cell. Accordingly, the invention further relates to a cell comprising said nucleic acid molecule or said vector. Such methods, for example, include the techniques described in Sambrook (1989), loc. cit. and Ausubel (1989), loc. cit. Accordingly, calcium chloride transfection or electroporation is commonly utilized for prokaryotic cells, whereas calcium phosphate treatment or electroporation may be used for other cellular hosts (Sambrook (1989), loc. cit.). As a further alternative, the nucleic acid molecules and vectors of the invention can be reconstituted into liposomes for delivery to target cells. The nucleic acid molecule or vector of the invention which is present in the host cell may either be integrated into the genome of the host cell or it may be maintained extra-chromosomally. Accordingly, the present invention also relates to a host cell comprising the nucleic acid molecule and/or the vector of this invention. Host cells for the expression of polypeptides are well known in the art and comprise prokaryotic cells as well as eukaryotic cells, e.g. E. coli cells, yeast cells, invertebrate cells, CHO cells, CHO-K1 cells, HEK 293 cells, Hela cells, COS-1 monkey cells, melanoma cells such as Bowes cells, mouse L-929 cells, 3T3 cell lines derived from Swiss, Balb-c or NIH mice, BHK or HaK hamster cell lines and the like.

In a further aspect, the present invention comprises methods for the preparation of the conjugates of the present invention as well as the biosynthetic random coil polypeptide (or segment thereof) or biologically active proteins provided herein and comprising culturing the (host) cell of this invention and isolating said random coil polypeptide (or segment thereof) or the conjugate or a biologically active protein from the culture as described herein. In general, the inventive random coil polypeptide (or segment thereof), the conjugate or biologically active protein comprising a random coil domain may be produced by recombinant DNA technology, e.g. by cultivating a cell comprising the described nucleic acid molecule or vectors which encode the inventive biologically active protein or random coil polypeptide (or segment thereof) and isolating said protein/polypeptide from the culture. The inventive biologically active protein or random coil polypeptide (or segment thereof) may be produced in any suitable cell culture system including prokaryotic cells, e.g. E. coli BL21, KS272 or JM83, or eukaryotic cells, e.g. Pichia pastoris, yeast strain X-33 or CHO cells. Further suitable cell lines known in the art are obtainable from cell line depositories like the American Type Culture Collection (ATCC).

The term “prokaryotic” is meant to include bacterial cells while the term “eukaryotic” is meant to include yeast, higher plant, insect and mammalian cells. The transformed hosts can be grown in fermentors and cultured according to techniques known in the art to achieve optimal cell growth. In a further embodiment, the present invention relates to a process for the preparation of a random coil polypeptide (or segment thereof) or a biologically active protein described above comprising cultivating a cell of the invention under conditions suitable for expression of the biologically active protein or random coil polypeptide (or segment thereof) and isolating said protein/polypeptide from the cell or the culture medium.

The random coil polypeptide (or segment thereof) per se of the present invention does, preferably not comprises any chemically reactive group, except for, possibly, one N-terminal primary (or, in the case of proline, secondary) amino group and one carboxylate group at the C-terminus of the polymer. However, it is evident for the skilled artisan that the biosynthetic random coil polypeptide/polymer as provided herein may comprise a chemically reactive group, for example when said random coil polypeptide/polymer is part of a “fusion protein”/“fusion construct”. As also described above, the biosynthetic random coil polypeptide (or segment thereof) can be prepared by recombinant expression in a transformed cell in several ways according to methods well known to the person skilled in the art, for example: (i) direct expression in the cytoplasm with the help of an N-terminal Met residue/start codon; (ii) secretion via an N-terminal signal peptide, for example OmpA, PhoA (Monteilhet (1993) Gene. 1993 125:223-228), mellitin (Tessier (1991) Gene 98: 177-183), interleukin 2 (Zhang (2005) J Gene Med 7: 354-365), hGH (Pecceu (1991) Gene 97(2):253-258) and the like, followed by intracellular cleavage resulting in the mature N-terminus, such as Ala or Pro; (iii) expression as a fusion protein with another soluble protein, e.g., maltose-binding protein at the N-terminus and with a protease cleavage site interspersed (Kapust and Waugh (2000) Protein Expr. Purif. 19:312-318), followed by specific protease cleavage in vitro or in vivo, thus releasing the amino acid polymer/polypeptide with its mature N-terminus such, as Ala or Pro. Another suitable fusion partner is the SUMO protein, which can be cleaved by SUMO protease, as described in Examples 20 and 21. Further fusion partners include, without limitation, glutathion-S-transferase, thioredoxin, a cellulose-binding domain, an albumin-binding domain, a fluorescent protein (such as GFP), protein A, protein G, an intein and the like (Malhotra (2009) Methods Enzymol. 463:239-258).

As explained above, the random coil polypeptides (or polypeptide segments)/polymers described consist predominantly of alanine and proline residues, whereas serine, threonine or asparagine, which are required for O- or N-glycosylation, are preferably absent. Thus, the production of the polypeptide itself or of a biologically active protein comprising the random coil polypeptide (or polypeptide segment thereof) or, generally, a fusion protein comprising the random coil polypeptide (or polypeptide segment thereof) surprisingly can result in a monodisperse product preferably devoid of post-translational modifications within the Pro-Ala sequence This is an advantage for recombinant protein production in eukaryotic cells, like chinese hamster ovarian cells (CHO) or yeast, which are often chosen for the biosynthesis of complex proteins. For example, yeast has been used for the production of approved therapeutic proteins such as insulin, granulocyte-macrophage colony stimulating factor, platelet-derived growth factor or hirudin (Gerngross (2004) Nat. Biotechnol. 22:1409-1414). CHO cells have served for the production of therapeutic proteins such as coagulation factor IX, interferone β-1a, tenecteplase (Chu (2001) Curr. Opin. Biotechnol. 12:180-187) or gonadotropins, where the glycocomponent may positively influence several aspects like functional activity, folding, dimerization, secretion as well as receptor interaction, signal transduction, and metabolic clearance (Walsh (2006) Nat. Biotechnol. 24:-1241-1252). Accordingly, the preparation of the inventive constructs, random coil polypeptides and conjugates in eukaryotic expression systems is also disclosed in context of the present invention.

With the means and methods provided herein it is now possible to manufacture and provide for the herein disclosed conjugates and molecules comprising (i) a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues and (ii) a further molecule of interest, like a useful protein, a protein segment or a small molecule. The present invention, therefore, also provides for methods for the preparation or manufacture of such conjugates as well as of biosynthetic random coil polypeptides and/or molecules or conjugates comprising the same. Accordingly, the present invention also provides for a method for the preparation and/or manufacture of a random coil polypeptide or a random coil polypeptide segment as comprised in the conjugates, like drug conjugates, food conjugates, diagnostic conjugates and the like. Also methods for the preparation and/or manufacture of the biologically active protein or conjugate comprising the random coil polypeptide or the random coil polypeptide segment are provided. Furthermore, methods for the preparation and/or manufacture and/or for the preparation and/or manufacture of a polypeptide that comprises or that is an amino acid sequence that has or that mediates a biological activity and that additionally comprises said random coil polypeptide or random coil polypeptide segment are provided. These methods, in particular comprise (as one step) the cultivation of the (host) cell as provided herein above and (as a further step) the isolation of said random coil polypeptide or biologically active protein and/or said biologically active protein and/or said polypeptide conjugate from the culture or from said cell. This isolated random coil, a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues as well as the isolated conjugate may than be further processed. For example, said biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues may be chemically linked or coupled to a molecule of interest, as also shown in the appended examples. Furthermore and as an alternative, the molecule of interest may be enzymatically conjugated e.g. via transglutaminase (Besheer (2009) J Pharm Sci. 98:4420-8) or other enzymes (Subul (2009) Org. Biomol. Chem. 7:3361-3371) to the said biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting of proline and alanine amino acid residues.

The random coil polypeptide (or segment thereof) and/or a protein conjugate comprising random coil polypeptide (or segment thereof) and a protein of interest, like a biologically or therapeutically active protein or a protein to be used in, e.g. diagnostic methods, can be isolated (inter alia) from the growth medium, cellular lysates, periplasm or cellular membrane fractions. (Again, the present invention is not limited to (protein) conjugates that are useful in a medical or pharmaceutical setting. The means and methods provided herein are also of use in other industrial areas, like, but not limited to food and beverage industry, nutrient industry, paper industry, bioreagent industry, research tool and reagent industry, industries where enzymes are to be used, cosmetic industry, oil processing and oil recovery, and the like). The isolation and purification of the expressed polypeptides of the invention may be performed by any conventional means (Scopes (1982) “Protein Purification”, Springer, New York, N.Y.), including ammonium sulphate precipitation, affinity purification, column chromatography, gel electrophoresis and the like and may involve the use of monoclonal or polyclonal antibodies directed, e.g., against a tag fused with the biologically active protein of the invention. For example, the protein can be purified via the Strep-tag II using streptavidin affinity chromatography (Skerra (2000) Methods Enzymol. 326:271-304) as described in the appended examples. Substantially pure polypeptides of at least about 90 to 95% homogeneity (on the protein level) are preferred, and 98 to 99% or more homogeneity are most preferred, in particular for pharmaceutical use/applications. Depending upon the host cell/organism employed in the production procedure, the polypeptides of the present invention may be glycosylated or may be non-glycosylated.

The invention further relates to the use of the biologically active protein, the random coil polypeptide (or segment thereof) or the conjugates, like the drug conjugates of the invention, the nucleic acid molecule of the invention, the vector of the invention or the (host) cell of the invention for the preparation of a medicament, wherein said biologically active protein or drug (or any other small molecule or protein of interest) has an increased in vivo and/or in vitro stability as compared to a control molecule that does not comprise or that is not linked to a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues.

In yet another embodiment, the present invention relates to a method for the treatment of diseases and/or disorders that benefit from the improved stability of said biologically active protein or drug, comprising administering the biologically active protein or drug conjugate as described herein to a mammal in need of such treatment. Depending on the biological activity of the inventive protein or drug conjugate, the skilled person is readily capable of determining which disease/disorder is to be treated with a specific biologically active protein or drug conjugate of the invention. Some non-limiting examples are listed in the following Table:

Biologically active protein (or a biologically active component/fragment Disorder/disease thereof) or drug to be treated granulocyte colony stimulating cancer and/or chemotherapy factor related neutropenia human growth hormone growth hormone deficiency related hypoglycaemia and/or growth failure interferon α cancer, viral infection, hepatitis C interferon β auto-immune disease, multiple sclerosis interferon γ viral infection tumor necrosis factor cancer interleukin-20 psoriasis α-galactosidase A Fabry disease myostatin antagonist sarcopenia gastric inhibitory polypeptide type 2 diabetes alpha-1 antitrypsin enzyme replacement therapy, cystic fibrosis, chronic obstructive pulmonary diseases, acute respiratory syndrome, severe asthma. erythropoietin anaemia coagulation factor VIII haemophilia gp120/gp160 HIV soluble tumor necrosis factor I inflammatory disease and II receptor reteplase thrombosis, myocardial infarction exendin-4 diabetes interleukin-1 receptor auto-immune disease, rheumatoid antagonist (IL-1ra; anakinra) arthritis interleukin-2 cancer insulin diabetes asparaginase acute lymphoblastic leukemia, non- Hodgkin's lymphoma onconase malignant mesothelioma and other types of cancer streptokinase thrombotic disorders neutrophil gelatinase- microbial infection, kidney associated lipocalin reperfusion injury antibodies and their fragments, immunological, oncological, including single domain neovascular, and infectious antibodies, single chain and diseases etc. other engineered fragments including CDR mimetic peptides and CDRs granulocyte-macrophage chemotherapy related neutropenia colony-stimulating factor follicle-stimulating hormone infertility glucocerebrosidase Gaucher's disease thymosin alpha 1 chronic hepatitis B, cancer glucagon hypoglycemia somatostatin acromegaly adenosine deaminase adenosine deaminase deficiency Interleukin-11 thrombocytopenia coagulation factor VIIa haemophilia coagulation factor IX hemophilia hematide anemia interferone λ hepatitis C leptin lipodystrophy, obesity, Alzheimer's disease, type I diabetes interleukin-22 receptor psoriasis subunit alpha (IL-22ra) interleukin 22 metastatic melanoma hyaluronidase solid tumors fibroblast growth factor 18 osteoarthritis fibroblast growth factor 21 diabetes type II, obesity, dyslipidemia, metabolic disorders glucagon-like peptide 1 diabetes osteoprotegerin cancer, osteoporosis, rheumatoid arthritis IL-18 binding protein rheumatoid arthritis growth hormone-releasing HIV-associated lipodystrophy factor soluble TACI receptor systemic lupus erythematosus, multiple sclerosis, rheumatoid arthritis thrombospondin-1 cancer soluble VEGF receptor Flt-1 cancer IL-4 mutein (IL-4 receptor asthma antagonist) cyclosporine organ rejection fumagillin cancer naltrexone alcohol dependence octreotide acromegaly, carcinoid tumors teduglutide short bowel syndrome, Crohn's disease goserelin advanced prostate cancer, breast cancer camptothecin cancer vancomycin Gram-positive pneumonias

In accordance with the above, the biologically active protein, the random coil polypeptide (or segment thereof), the drug conjugate, the nucleic acid, the vector or the cell may be used for the preparation of a medicament which preferably has or confers an increased in vivo and/or in vitro stability, in particular for the biologically active protein and/or drug component, for the treatment of hormone deficiencies or related disorders, auto-immune disease, cancer, anaemia, neovascular diseases, infectious/inflammatory diseases, thrombosis, myocardial infarction, diabetes, infertility, Gaucher's disease, hepatitis, hypoglycaemia, acromegaly, adenosine deaminase deficiency, thrombocytopenia, haemophilia, anemia, obesity, Alzheimer's disease, lipodistrophy, psoriasis, metastatic melanoma, osteoarthritis, dyslipidemia, rheumatoid arthritis, systemic lupus erythromatosis, multiple sclerosis, asthma, osteoporosis, and reperfusion injury or other kidney diseases, for example. In one embodiment, the biologically active protein, the drug conjugate the nucleic acid, the vector or the cell is for the use as a medicament which has an increased in vivo and/or in vitro stability of said biologically active protein/drug conjugate. Similarly, the biologically active protein, the random coil polypeptide (or segment thereof), the drug conjugate, the nucleic acid, the vector or the cell are for use in the treatment of for the treatment of hormone deficiencies or related disorders, auto-immune disease, proliferative disorders, like cancer, anaemia, neovascular diseases, infectious and/or inflammatory diseases, thrombosis, myocardial infarction stroke, diabetes, infertility, penile dysfunction, Gaucher's disease, Fabry disease, sarcopenia, cystic fibrosis, obstructive pulmonary diseases, acute respiratory syndrome, hepatitis, hypoglycaemia, acromegaly, adenosine deaminase deficiency, thrombocytopenia, haemophilia, anemia, obesity, Alzheimer's disease, lipodistrophy, psoriasis, metastatic melanoma, osteoarthritis, dyslipidemia, rheumatoid arthritis, systemic lupus erythromatosis, multiple sclerosis, asthma, osteoporosis, and reperfusion injury or other kidney diseases, for example.

The present invention also relates to the use of the nucleic acid molecules, vectors as well as transfected cells as provided herein and comprising the nucleic acid molecules or vectors of the present invention in medical approaches, like, e.g. cell based gene therapy approaches or nucleic acid based gene therapy approaches.

In a further embodiment, the random coil polypeptide (or polypeptide segment thereof) as provided herein, the biologically active, heterologous protein/protein construct or the drug or food conjugate or other conjugates that comprise the biosynthetic random coil polypeptide (or polypeptide segment thereof) and/or the nucleic acid molecule or the vector or the host cell of the present invention) is part of a composition. Said composition may comprise one or more of the inventive random coil polypeptides (or polypeptide segments thereof), biologically active proteins, food conjugates, conjugates of interest, drug conjugates or nucleic acid molecules, vectors and/or host cells encoding and/or expressing the same. Said composition may be a pharmaceutical composition, optionally further comprising a pharmaceutically acceptable carrier and/or diluent. In a further embodiment, the present invention relates to the use of the herein described biologically active protein, the random coil polypeptide (or segment thereof) or the drug conjugate for the preparation of a pharmaceutical composition for the prevention, treatment or amelioration of diseases which require the uptake of such a pharmaceutical composition.

As mentioned herein above, not only the herein disclosed conjugates, like drug conjugates or diagnostic conjugates, and/or biologically active, heterologous proteins/protein constructs (comprising the inventive random coil polypeptide or polypeptide segment thereof) are in particular of medical or pharmaceutical use. Also said random coil polypeptide or polypeptide segment may be per se employed in such a medical context, for example as “plasma expander” or as blood surrogate, in the amelioration, prevention and/or treatment of a disorder related to an impaired blood plasma amount or blood plasma content or in the amelioration, prevention and/or treatment of a disorder related to an impaired blood volume. Disorders that are treated with plasma expanders are, but not limited to, disorders affiliated with blood loss, like injuries, surgeries, burns, trauma, or abdominal emergencies, infections, dehydratations etc. Yet, such a medical use is not limited to the random coil polypeptide or polypeptide segment of this invention but can also be extended to certain drug conjugates as disclosed herein or even to certain biologically active, heterologous proteins/protein constructs.

In one embodiment, the composition as described herein may be a diagnostic composition, for example an imaging reagent, optionally further comprising suitable means for detection, wherein said diagnostic composition has an increased in vivo and/or in vitro stability.

The compositions of the invention may be in solid or liquid form and may be, inter alia, in a form of (a) powder(s), (a) tablet(s), (a) solution(s) or (an) aerosol(s). Furthermore, it is envisaged that the medicament of the invention might comprise further biologically active agents, depending on the intended use of the pharmaceutical composition.

Administration of the suitable (pharmaceutical) compositions may be effected by different ways, e.g., by parenteral, subcutaneous, intravenous, intraarterial, intraperitoneal, topical, intrabronchial, intrapulmonary and intranasal administration and, if desired for local treatment, intralesional administration. Parenteral administrations include intraperitoneal, intramuscular, intradermal, subcutaneous, intravenous or intraarterial administration. The compositions of the invention may also be administered directly to the target site, e.g., by biolistic delivery to an external or internal target site, like a specifically effected organ.

Examples of suitable pharmaceutical carriers, excipients and/or diluents are well known in the art and include phosphate buffered saline solutions or other buffer solutions, water, emulsions, such as oil/water emulsions, various types of wetting agents, sterile solutions etc. Compositions comprising such carriers can be formulated by well known conventional methods. Suitable carriers may comprise any material which, when combined with the biologically active protein/drug conjugate of the invention, retains its biological and/or pharmaceutical activity (see Remington's Pharmaceutical Sciences (1980) 16th edition, Osol, A. Ed, Mack Publishing Company, Easton, Pa.). Preparations for parenteral administration may include sterile aqueous or non-aqueous solutions, suspensions, and emulsions. The buffers, solvents and/or excipients as employed in context of the pharmaceutical composition are preferably “physiological” as defined herein above. Examples of non-aqueous solvents are propylene glycol, polyethylene glycol, vegetable oils such as olive oil, and injectable organic esters such as ethyl oleate. Aqueous carriers include water, alcoholic/aqueous solutions, emulsions or suspensions, including saline and buffered media. Parenteral vehicles may include sodium chloride solution, Ringer's dextrose, dextrose and sodium chloride, lactated Ringer's, or fixed oils. Intravenous vehicles may include fluid and nutrient replenishes, electrolyte replenishers (such as those based on Ringer's dextrose), and the like. Preservatives and other additives may also be present, including antimicrobials, anti-oxidants, chelating agents and/or inert gases and the like. In addition, a pharmaceutical composition of the present invention might comprise proteinaceous carriers, like, e.g., serum albumin or immunoglobulin, preferably of human origin.

These pharmaceutical compositions can be administered to the subject at a suitable dose. The dosage regimen will be determined by the attending physician and clinical factors. As is well known in the medical arts, dosages for any one patient depend upon many factors, including the patient's size, body surface area, age, the particular compound to be administered, sex, time and route of administration, general health, and other drugs being administered concurrently. Pharmaceutically active matter may be present in amounts between 1 μg and 20 mg/kg body weight per dose, e.g. between 0.1 mg to 10 mg/kg body weight, e.g. between 0.5 mg to 5 mg/kg body weight. If the regimen is a continuous infusion, it should also be in the range of 1 μg to 10 mg per kilogram of body weight per minute. Yet, doses below or above the indicated exemplary ranges also are envisioned, especially considering the aforementioned factors.

Furthermore, it is envisaged that the pharmaceutical composition of the invention might comprise further biologically or pharmaceutically active agents, depending on the intended use of the pharmaceutical composition. These further biologically or pharmaceutically active agents may be e.g. antibodies, antibody fragments, hormones, growth factors, enzymes, binding molecules, cytokines, chemokines, nucleic acid molecules and drugs.

It is of note that the present invention is not limited to pharmaceutical compositions. Also compositions to be used in research or as diagnostic(s) are envisaged. It is, for example, envisaged that the biologically active proteins or drug conjugates comprising a random coil domain or component as defined herein, are used in a diagnostic setting. For such a purpose, the inventive biologically active protein or drug conjugate of this invention may be labelled in order to allow detection. Such labels comprise, but are not limited to, radioactive labels (like [³H]hydrogen [¹²⁵I]iodide or [¹²³I]iodide), fluorescent labels (including fluorescent proteins, like green fluorescent protein (GFP) or fluorophores, like fluorescein isothiocyanate (FITC)) or NMR labels (like gadolinium chelates). The here defined labels or markers are in no way limiting and merely represent illustrative examples. The diagnostic compositions of this invention are particularly useful in tracing or imaging experiments or in a diagnostic medicals setting. In the appended Examples and Figures, the preparation of a corresponding construct is provided that comprises conjugates comprising (i) a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, and (ii) fluorescein or digoxigenin; see appended FIGS. 13 and 14 and the corresponding figure legend as well as illustrative Example 22.

But not only pharmaceutical or diagnostic uses of the means and methods provided herein are within the gist of the present invention. The compounds/conjugates provided herein are also useful in certain other industrial areas, like in the food industry, the beverage industry, the cosmetic industry, the oil industry, the paper industry and the like. Therefore, the present invention also provides for uses of the biosynthetic random coil polypeptide as provided herein in such industrial areas. Also part of this invention is, accordingly, a method for the production of a cosmetic, of a compound to be used in cosmetic treatments, of a food or of a beverage, said method comprising the culture of the cell comprising a nucleic acid molecule (or a vector) encoding a random coil polypeptide as defined herein or encoding a biologically active protein and/or a biologically active protein and/or a polypeptide that comprises or that is an amino acid sequence that has or that mediates an activity. Such a method also includes the isolation of said random coil polypeptide, said biologically active protein and/or said biologically active protein or said polypeptide that comprises or that is an amino acid sequence that has or that mediates an activity, like a biological activity, and that additionally comprises said random coil polypeptide or random coil polypeptide segment from the culture or from said cell. In the same context, other conjugates of interest can be produced, for example conjugates which are useful in different areas of industry, like in the oil or paper industry. The person skilled in the art is readily in a position to adapt the herein provided means and methods for the generation of corresponding molecular/recombinant constructs as well as for the generation of conjugates that comprise a biosynthetic random coil polypeptide or polypeptide segment comprising an amino acid sequence consisting solely of proline and alanine amino acid residues, wherein said amino acid sequence consists of at least 50 proline (Pro) and alanine (Ala) amino acid residues, and a small molecule or a polypeptide of interest.

In yet another embodiment, the present invention provides for a kit comprising the random coil polypeptide (or polypeptide segment thereof), the biologically active protein, the drug conjugate, the nucleic acid molecule encoding said biologically active protein encoding said biologically active protein and/or encoding said biologically active protein and/or encoding said polypeptide that comprises or that is an amino acid sequence that has or that mediates an activity (for example a biological activity), the vector comprising said nucleic acid molecule or the cell comprising said nucleic acid or said vector as described herein. The kit of the present invention may further comprise, (a) buffer(s), storage solutions and/or additional reagents or materials required for the conduct of medical, scientific or diagnostic assays and purposes. Furthermore, parts of the kit of the invention can be packaged individually in vials or bottles or in combination in containers or multicontainer units.

The kit of the present invention may be advantageously used, inter alia, for carrying out the method of the invention and could be employed in a variety of applications referred herein, e.g., as diagnostic kits, as research tools or as medical tools. Additionally, the kit of the invention may contain means for detection suitable for scientific, medical and/or diagnostic purposes. The manufacture of the kits preferably follows standard procedures which are known to the person skilled in the art.

The invention is further illustrated by the following, non-limiting Figures and Examples.

FIG. 1. Gene design for the PA #1 Pro/Ala polymer/polypeptide sequence.

Nucleotide and encoded amino acid sequence of a building block for PA #1 (SEQ ID NO: 1) obtained by hybridization of two complementary oligodeoxynucleotides (upper/coding strand oligodeoxynucleotide SEQ ID NO: 17, lower/non-coding strand oligodeoxynucleotide SEQ ID NO: 18). The resulting nucleic acid has two sticky ends (shown in lower case letters), corresponding to an Ala codon and anti-codon, respectively, and are mutually compatible. Upon repeated ligation of such a building block, concatamers encoding Pro-Ala polypeptides of varying lengths can be obtained and subsequently cloned, for example, via (a) SapI restriction site(s).

FIG. 2. Cloning strategies for a Pro/Ala polymer/polypeptide sequence as fusion to a Fab fragment or to human IFNa2b.

(A) Nucleotide and encoded amino acid sequence stretch (upper/coding strand SEQ ID NO: 19, lower/non-coding strand SEQ ID NO: 20, encoded amino acid sequence SEQ ID NO: 21) around the C-terminus of the immunoglobulin light chain of an antibody Fab fragment as encoded on pASK88-Fab-2×SapI (SEQ ID NO: 22), a derivative of pASK75, used for subcloning of Pro/Ala polymer/polypeptide sequences and expression of corresponding biologically active proteins. The nucleotide sequence carries two SapI recognition sites in mutually reverse orientation, which leads upon digest to protruding DNA ends that are compatible with the synthetic gene cassette shown in FIG. 1. The recognition sequences and the C-terminal amino acids of the light chain are underlined.

(B) Nucleotide sequence and encoded amino acid sequence (upper/coding strand SEQ ID NO: 23, lower/non-coding strand SEQ ID NO: 24, encoded amino acid sequence SEQ ID NO: 25) of a PA #1 polymer/polypeptide with 20 residues after insertion of a single cassette as shown in FIG. 1 into the pASK88-Fab-2×SapI plasmid. Similar ligation/insertion of 10 such repeated cassettes resulted in the plasmid vector pFab-PA #1(200) (Seq ID NO: 28) coding for a polymer/polypeptide with 200 residues (SEQ ID NO: 26 and 27). The SapI restriction sites flanking the Pro/Ala polymer-encoding sequence are labelled (recognition sequences are underlined).

(C) Plasmid map of pFab-PA #1(200) (SEQ ID NO: 28). The structural genes for the heavy chain (HC) and light chain (LC) of the Fab-PA #1(200) are under transcriptional control of the tetracycline promoter/operator (tet^(p/o)) and the operon ends with the lipoprotein terminator (t_(lpp)). HC comprises the bacterial OmpA signal peptide, the variable (VH) and the first human IgG1 heavy chain constant C domain (CH) as well as the His₆-tag. LC comprises the bacterial PhoA signal peptide, the variable (VL) and human light chain constant (CL) domain, the PA #1 polymer/polypeptide with 200 residues. The plasmid backbone of pFab-PA #1(200) outside the expression cassette flanked by the XbaI and HindIII restriction sites is identical with that of the generic cloning and expression vector pASK75 (Skerra (1994) Gene 151:131-135). Singular restriction sites are indicated.

(D) Nucleotide and amino acid sequence stretch (upper/coding strand SEQ ID NO: 29, lower/non-coding strand SEQ ID NO: 30, encoded amino acid sequence SEQ ID NO: 31) around the N-terminus of human IFNa2b as cloned on pASK-IFNa2b (SEQ ID NO: 32). The single restriction site SapI that can be used for insertion of the Pro/Ala polymer-encoding sequence is labelled (recognition sequence is underlined). The two C-terminal amino acids of the Strep-tag II are underlined. The first amino acid of the mature IFNa2b is labelled with +1.

(E) Nucleotide and encoded amino acid sequence stretch (upper/coding strand SEQ ID NO: 33, lower/non-coding strand SEQ ID NO: 34, encoded amino acid sequence SEQ ID NO: 35) of the N-terminus of IFNa2b after insertion of one PA #1 polymer sequence cassette as shown in FIG. 1. The single restriction site SapI, that remains after insertion of the Pro/Ala polymer-encoding sequence, is labelled (recognition sequences are underlined). The first amino acid of IFNa2b as part of the fusion protein is labelled (1) and the two C-terminal amino acids of the Strep-tag II are underlined. Similar ligation/insertion of 10 repeated PA #1 polymer sequence cassettes resulted in the plasmid vector pPA #1(200)-IFNa2b coding for a polymer/polypeptide with 200 residues (SEQ ID NO: 36)

(F) Plasmid map of pPA #1(200)-IFNa2b (SEQ ID NO: 37). The structural gene for biologically active protein PA #1(200)-IFNa2b (comprising the bacterial OmpA signal peptide, the Strep-tag II, the PA #1 polymer/polypeptide segment with 200 residues, and human IFNa2b) is under transcriptional control of the tetracycline promoter/operator (tet^(p/o)) and ends with the lipoprotein terminator (t_(lpp)). The plasmid backbone outside the expression cassette flanked by the XbaI and HindIII restriction sites is identical with that of the generic cloning and expression vector pASK75 (Skerra (1994) loc. cit.). Singular restriction sites are indicated.

FIG. 3. Analysis of the purified recombinant Fab fragment and the purified recombinant IFNa2b as well as their Pro/Ala polypeptide/polymer fusions by SDS-PAGE.

The recombinant proteins were produced in E. coli KS272 (Strauch (1988) Proc. Natl. Acad. Sci. USA 85:1576-80) via periplasmic secretion and purified by means of the His₆-tag (Fab) or the Strep-tag II (IFNa2b) using immobilized metal or streptavidin affinity chromatography, respectively.

(A) Analysis of the purified recombinant Fab and its PA #1 fusion with 200 residues by 12% SDS-PAGE. The gel shows 2 μg protein samples each of Fab and Fab-PA #1(200). Samples on the left were reduced with 2-mercaptoethanol whereas repeated samples on the right were left unreduced. Sizes of protein markers—applied under reducing conditions—are indicated on the left margin. Upon reduction of the interchain disulfide bridge the Fab fragment and its 200 residue PA #1 fusion appear as two homogenous bands. In the case of the reduced Fab fragment, the two bands with molecular sizes of ca. 24 and 26 kDa, respectively, correspond to the separated LC and HC. In the case of the reduced Fab-PA #1(200) fusion protein the band at 24 kDa corresponds to the HC, whereas the band at ca. 90 kDa corresponds to the LC fused with the PA #1(200) polypeptide segment. Under non-reducing conditions, the Fab fragment and its PA #1(200) fusion appear as single homogeneous bands with apparent molecular sizes of ca. 45 kDa and 100 kDa, respectively. The two apparent size values for the Fab-PA #1(200) fusion protein are significantly larger than the calculated masses of 64.3 kDa for the non-reduced Fab-PA #1(200) and of 39.1 kDa for the isolated LC-PA #1(200). This effect is due to the addition of the Pro/Ala polymer/polypeptide segment because the Fab fragment itself, with a calculated mass of 48.0 kDa, or its unfused light chain exhibit essentially normal electrophoretic mobility.

(B) Analysis of the purified recombinant IFNa2b and its PA #1 fusion protein with 200 residues by 12% SDS-PAGE. The gel shows 2 μg protein samples each of IFNa2b and of PA #1(200)-IFNa2b. Samples on the left were reduced with 2-mercaptoethanol whereas corresponding samples on the right were left unreduced. Sizes of protein markers—applied under reducing conditions—are indicated on the left margin. The two proteins appear as single homogeneous bands with apparent molecular sizes of ca. 20 kDa and ca. 80 kDa in the reduced form. The latter value is significantly larger than the calculated mass of 37.0 kDa for PA #1(200)-IFNa2b. This effect is due to the addition of the Pro/Ala polymer/polypeptide segment because the IFNa2b itself, with a calculated mass of 20.9 kDa, exhibits essentially normal electrophoretic mobility. IFNa2b in the non-reduced state has a slightly higher electrophoretic mobility, indicating a more compact form as a result of its two intramolecular disulfide bridges.

FIG. 4. Quantitative analysis of the hydrodynamic volumes of the purified recombinant Fab and IFNa2b as well as their PA #1(200) fusions.

(A) Analytical size exclusion chromatography (SEC) of Fab and Fab-PA #1(200). 250 μl of the purified protein at a concentration of 0.25 mg/ml was applied to a Superdex S200 10/300 GL column equilibrated with PBS buffer. Absorption at 280 nm was monitored and the peak of each chromatography run was normalized to a value of 1. The arrow indicates the void volume of the column (7.8 ml).

(B) Calibration curve for the chromatograms from (A) using a Superdex S200 10/300 GL column. The logarithm of the molecular weight (MW) of marker proteins (cytochrome c, 12.4 kDa; carbonic anhydrase, 29.0 kDa; ovalbumin, 43.0 kDa; bovine serum albumin, 66.3 kDa; alcohol dehydrogenase, 150 kDa, β-amylase, 200 kDa, apo-ferritin, 440 kDa) was plotted vs. their elution volumes (black circles) and fitted by a straight line. From the observed elution volumes of the Fab fragment and its PA #1 fusion protein (black squares) their apparent molecular sizes were determined as follows. Fab: 31 kDa (true mass: 48.0 kDa); Fab-PA #1(200): 237 kDa (true mass: 64.3 kDa). These data show that fusion with the PA #1 polypeptide confers a much enlarged hydrodynamic volume.

(C) Analytical size exclusion chromatography of IFNa2b and PA #1(200)-IFNa2b. 250 μl of each purified protein at a concentration of 0.25 mg/ml was applied to a Superdex S200 10/300 GL column equilibrated with phosphate-buffered saline, PBS. Absorption at 280 nm was monitored and the peak of each chromatography run was normalized to a value of 1. The arrow indicates the void volume of the column (7.8 ml).

(D) Calibration curve for the chromatogram from (C) using a Superdex S200 10/300 GL column. The logarithm of the molecular weight (MW) of marker proteins (see B) was plotted vs. their elution volumes (black circles) and fitted by a straight line. From the observed elution volumes of IFNa2b and its PA #1 fusion protein (black squares) their apparent molecular sizes were determined as follows. IFNa2b: 22.5 kDa (true mass: 20.9 kDa); PA #1(200)-IFNa2b: 229.0 kDa (true mass: 37.0 kDa). These data show that fusion with the PA #1 polypeptide confers a much enlarged hydrodynamic volume.

FIG. 5. Experimental secondary structure analysis of recombinant proteins and their PA #1 polymer/polypeptide fusions by circular dichroism (CD) spectroscopy.

Spectra were recorded at room temperature in 50 mM K₂SO₄, 20 mM K-phosphate pH 7.5 and normalized to the molar ellipticity, Θ_(M), for each protein.

(A) CD spectra of the purified recombinant Fab and Fab-PA #1(200). The CD spectrum for the Fab fragment shows the typical features of a predominant β-sheet protein with a broad negative maximum around 216 nm (Sreerama in: Circular Dichroism—Principles and Applications (2000) Berova, Nakanishi and Woody (Eds.) Wiley, New York, N.Y., pp. 601-620), which indicates the correct folding of the bacterially produced Fab fragment. The spectrum of its fusion protein with the Pro/Ala polymer/polypeptide reveals a dominant negative band below 200 nm, which is indicative of random coil conformation. In addition, there is a shoulder around 220 nm, which results from the β-sheet contribution of the Fab fragment and indicates its correct folding even as part of the fusion protein.

(B) Molar difference CD spectrum for Fab-PA #1(200) obtained by subtraction of the spectrum for the Fab fragment. The difference CD spectrum represents the secondary structure of the 200 residue PA #1 polymer/polypeptide segment and reveals a strong minimum around 200 nm, which is a clear indication of random coil conformation in the buffered aqueous solution (Greenfield (1969) Biochemistry 8: 4108-4116; Sreerama (2000) loc. cit.; Fändrich (2002) EMBO J. 21:5682-5690).

(C) CD spectra of the purified recombinant IFNa2b and PA #1(200)-IFNa2b. The CD spectrum for IFNa2b shows the typical features of a predominant α-helix protein with two negative bands around 208 nm and 220 nm (Sreerama (2000) loc. cit.), which indicates the correct folding of the bacterially produced human IFNa2b. The spectrum of its fusion protein with the Pro/Ala polymer/polypeptide reveals characteristic deviations with a dominant minimum around 200 nm, which is indicative of random coil conformation. In addition, there is a shoulder around 220 nm, which results from the a-helical contribution of IFNa2b and indicates the correct folding of the IFNa2b even as part of the fusion protein.

(D) Molar difference CD spectrum for PA #1(200)-IFNa2b obtained by subtraction of the spectrum for IFNa2b. The difference CD spectrum represents the secondary structure of the 200 residue PA #1 polymer/polypeptide segment and reveals a strong minimum around 200 nm, essentially identical to the one shown in (B). This is again a clear indication of random coil conformation in buffered aqueous solution for a biological polymer comprising Pro and Ala residues according to the invention.

FIG. 6. Secretory production of a fusion protein between human growth hormone (hGH) and the genetically encoded PA #1 polymer in CHO cells.

(A) Nucleotide and amino acid sequence stretch (upper/coding strand SEQ ID NO: 38, lower/non-coding strand SEQ ID NO: 39, encoded amino acid sequence SEQ ID NO: 40) around the N-terminus of hGH as cloned on pASK75-His6-hGH (SEQ ID NO: 41). The single restriction sites NheI, that can be used together with HindIII (not shown) for subcloning, and SapI, that can be used for insertion of the Pro/Ala polymer-encoding sequence, are labelled (recognition sequence is underlined). The six amino acids of the His6-tag are underlined. The first amino acid of the hGH is labelled with +1.

(B) Nucleotide and encoded amino acid sequence (upper/coding strand SEQ ID NO: 42, lower/non-coding strand SEQ ID NO: 43, encoded amino acid sequence SEQ ID NO: 44) of the N-terminus of hGH after insertion of one PA #1 polymer sequence cassette as shown in FIG. 1. The single restriction sites NheI, that can be used for subcloning, and SapI, that remains after insertion of the Pro/Ala polymer-encoding sequence, is labelled (recognition sequences are underlined). The first amino acid of hGH as part of the fusion protein is labelled (1) and the amino acids of the His6-tag are underlined. Similar ligation/insertion of 10 repeated PA #1 polymer sequence cassettes resulted in the plasmid vector pASK75-His6-PA #1(200)-hGH coding for the mature fusion protein SEQ ID NO: 45.)

(C) Plasmid map of pASK75-His6-PA #1(200)-hGH (SEQ ID NO: 46). The structural gene for biologically active protein His6-PA #1(200)-hGH (comprising the bacterial OmpA signal peptide, the His6-tag, the PA #1 polymer/polypeptide segment with 200 residues, and human GH) is under transcriptional control of the tetracycline promoter/operator (tet^(p/o)) and ends with the lipoprotein terminator (t_(lpp)). The plasmid backbone outside the expression cassette flanked by the XbaI and HindIII restriction sites is identical with that of the generic cloning and expression vector pASK75 (Skerra (1994) loc. cit.). Singular restriction sites are indicated.

(D) Plasmid map of pCHO-PA #1(200)-hGH, which encodes a His6-PA #1(200)-hGH fusion protein (SEQ ID NO: 47). The structural gene, comprising the human growth hormone signal peptide (Sp), the His₆-tag, the PA #1 polymer/polypeptide sequence with 200 residues (PA #1(200)), the human growth hormone (hGH), and containing the bovine growth hormone polyadenylation signal (bGH pA), is under transcriptional control of the cytomegalus virus promoter (CMV^(p)). The singular restriction sites NheI and HindIII are indicated. The resistance gene for neomycinphosphotransferase (neo) is under control of the SV40 promotor (SV40^(p)) and followed by a SV40 polyadenylation signal (SV40 pA). In addition, the plasmid contains the bacterial ColE1 origin of replication (ColE1-ori), the bacteriophage f1 origin of replication (f1-ori), and the β-lactamase gene (bla) to allow propagation and selection in E. coli.

(E) Western blot analysis of a fusion protein between hGH and the genetically encoded PA #1 polymer of 200 residues produced in CHO cells compared with recombinant hGH. CHO-K1 cells were transfected either with pCHO-PA #1(200)-hGH (SEQ ID NO: 48) or with pCHO-hGH (SEQ ID NO: 49), a similar plasmid encoding hGH without the PA #1(200) sequence (but also carrying the His6-tag). Two days after transfection, a sample of the cell culture supernatant was subjected to SDS-PAGE and Western blotting with an anti-hGH antibody conjugated with horse radish peroxidase. The two proteins appear as single bands indicated by arrows, with apparent molecular sizes of ca. 23 kDa (His6-hGH) and ca. 90 kDa (His6-PA #1-hGH). There is also a weak band around 60 kDa arising from serum proteins in the culture medium. Whereas the His6-tagged hGH appears at the calculated mass of 23.5 kDa, the apparent molecular size of His6-PA #1-hGH is significantly larger than its calculated mass of 39.5 kDa. This effect is due to the hydrophilic random coil nature of the Pro-Ala polymer.

FIG. 7. Theoretical prediction of secondary structure for the PA #1 Pro/Ala polypeptide/polymer sequence.

This illustration shows the output from the CHOFAS computer algorithm according to the Chou-Fasman method (Chou and Fasman (1974) Biochemistry 13: 222-245) as implemented on the Sequence Comparison and Secondary Structure prediction server at the University of Virginia. To avoid boundary effects at the amino and carboxy termini, the 20mer amino acid repeat according to FIG. 1 was pasted in three consecutive copies (resulting in a concatamer similar as encoded after repeated ligation/insertion of the synthetic gene cassette) and only the output for the central 20mer sequence block (boxed) was considered. In the case of the PA #1 polypeptide sequence/segment (SEQ ID NO: 1) the Chou-Fasman algorithm predicts 100% α-helical secondary structure. This is in contrast with the experimentally observed predominant random coil conformation for the PA #1 polypeptide/polypeptide segment as part of a fusion protein (see FIG. 5B/D).

FIG. 8: Quantitative analysis of the pharmacokinetics of the purified recombinant Fab fragment and its PA #1 polymer fusions with 200 and 600 residues in BALB/c mice.

Plasma samples from Example 16 were assayed for Fab, Fab-PA #1(200), and Fab-PA #1(600) concentrations using a sandwich ELISA. To estimate the plasma half-life of Fab, Fab-PA #1(200), and Fab-PA #1(600), the measured concentration values were plotted against time post intravenous injection and numerically fitted assuming a bi-exponential decay. The unfused Fab fragment exhibited a very fast clearance with an elimination half-life of 1.3±0.1 h. In contrast, the elimination phase determined for Fab-PA #1(200) and Fab-PA #1(600) was significantly slower, with terminal half-lives of 4.1±1.8 h and 38.8±11.2 h, respectively, thus demonstrating a ca. 3-fold and a ca. 30-fold prolonged circulation due to the Pro/Ala polymer fusion with 200 or 600 residues compared with the unfused Fab fragment.

FIG. 9: Analysis of the purified recombinant Fab fragment as fusion with the P1A1 or P1A3 polymer having 200 residues.

The recombinant proteins were produced in E. coli KS272 via periplasmic secretion and purified by means of the His₆-tag using immobilized metal affinity chromatography. The purified proteins were analyzed by 12% SDS-PAGE. The gel shows 2 μg protein samples each of Fab-P1A1(200) and Fab-P1A3(200) as well as, for comparison, of the unfused Fab fragment (cf. FIG. 3A). Samples on the left were reduced with 2-mercaptoethanol whereas analogous samples on the right were left unreduced. Sizes of protein markers—applied under reducing conditions—are indicated on the left margin. After reduction of the interchain disulfide bridges the Fab fragment and its 200 residue Pro/Ala fusions appear as two homogeneous bands. In the case of the reduced Fab fragment, the two bands with molecular sizes of ca. 24 and 26 kDa, respectively, correspond to the separated light chain (LC) and heavy chain fragment (HC). In the case of the reduced Fab-P1A1(200) fusion protein the band at 24 kDa corresponds to the HC, whereas the band at ca. 90 kDa corresponds to the LC fused with the P1A1(200) polypeptide. In the case of the reduced Fab-P1A3(200) fusion protein the band at 24 kDa corresponds to the HC, whereas the band at ca. 75 kDa corresponds to the LC fused with the P1A5(200) polypeptide. Under non-reducing conditions, the Fab fragment, its P1A1(200) and its P1A3(200) fusion appear as single prominent bands with apparent molecular sizes of ca. 45 kDa, 110 kDa, and 90 kDa, respectively. The apparent sizes for the Fab-P1A1(200) and Fab-P1A3(200) fusion proteins are significantly larger than the calculated masses of 65.3 kDa for the non-reduced Fab-P1A1(200) and of 64.0 kDa for the non-reduced Fab-P1A3(200). Also, the apparent sizes for the corresponding reduced light chains are significantly larger than the calculated masses of 40.7 kDa for the P1A1(200) LC and of 39.4 kDa for the P1A3(200) LC. This effect is due to the addition of the Pro/Ala polymer/polypeptide segment because the Fab fragment itself, with a calculated mass of 48.0 kDa, or its unfused light chain, with a calculated mass of 23.4 kDa, exhibit essentially normal electrophoretic mobility.

FIG. 10. Quantitative analysis of the hydrodynamic volumes of the purified recombinant Fab-P1A1(200) and Fab-P1A3(200) fusion proteins.

Analytical size exclusion chromatography (SEC) of Fab-P1A1(200) and Fab-P1A3(200). 250 μl of the purified protein at a concentration of 0.25 mg/ml was applied to a Superdex S200 10/300 GL column equilibrated with PBS. Absorption at 280 nm was monitored and the peak of each chromatography run was normalized to a value of 1. The arrow indicates the void volume of the column (7.8 ml). From the observed elution volumes of the fusion proteins their apparent molecular sizes were determined using a similar calibration curve as shown in FIG. 4B as follows. Fab-P1A1(200): 180.7 kDa (true mass: 65.3 kDa); Fab-P1A3(200): 160.2 kDa (true mass: 64.0 kDa). These data show that fusion of a protein with the P1A1 and/or P1A5 polypeptide confers a much enlarged hydrodynamic volume.

FIG. 11. Experimental secondary structure analysis of Fab-P1A1(200) and Fab-P1A3(200) fusions by circular dichroism (CD) spectroscopy.

Spectra were recorded at room temperature in 50 mM K₂SO₄, 20 mM K-phosphate pH 7.5 and normalized to the molar ellipticity, Θ_(M), for each protein.

(A) CD spectra of the purified recombinant Fab-P1A1(200) and Fab-P1A3(200). The CD spectra of the Fab fusion proteins with both Pro/Ala polymers/polypeptides each reveal a dominant negative band below 200 nm, which is indicative of random coil conformation. In addition, there is a shoulder around 220 nm, which arises from the β-sheet contribution of the Fab fragment and indicates its correct folding even as part of the fusion protein.

(B) Molar difference CD spectra for Fab-P1A1(200) and Fab-P1A3 (200) obtained by subtraction of the spectrum for the unfused Fab fragment (see FIG. 5A). The difference CD spectra represent the secondary structures of the 200 residue P1A1 (SEQ ID NO: 51) and P1A3 (SEQ ID NO: 3) polymers/polypeptide segments, respectively, and reveal a strong minimum around 200 nm, which is a clear indication of their random coil conformation in the buffered aqueous solution (Greenfield (1969) Biochemistry 8: 4108-4116; Sreerama (2000) loc. cit.; Fändrich (2002) EMBO J. 21:5682-5690).

FIG. 12: Preparation of an isolated biosynthetic Pro/Ala polymer/polypeptide.

(A) Plasmid map of pSUMO-PA #1(200) (SEQ ID NO: 60). The structural gene for the fusion protein MK-His(6)-SUMO-PA #1(200) comprising a start methionine codon followed by a lysine codon, an N-terminal affinity tag of six consecutive His residues, the cleavable small ubiquitin-like modifier (SUMO) protein Smt3p (Panavas (2009) Methods Mol Biol. 497: 303-17), and the PA #1 polymer/polypeptide segment with 200 residues (SEQ ID NO: 60) is under transcriptional control of the gene 10 promoter of the bacteriophage T7 and ends with the tϕ terminator. Additional plasmid elements comprise the origin of replication (ori), the ampicillin resistance gene (bla), and the f1 origin of replication. The plasmid backbone outside the expression cassette flanked by the NdeI and HindIII restriction sites is, except for a SapI restriction site that was eliminated by silent mutation, identical with that of the generic cloning and expression vector pRSET5a (Schoepfer (1993) 124: 83-85).

SEQ ID NO: 60 is provided in the enclosed sequence listing (which is also part of this description and specification) and is reproduced herein below.

gcacttttcg gggaaatgtg cgcggaaccc ctatttgttt atttttctaa atacattcaa 60 atatgtatcc gctcatgaga caataaccct gataaatgct tcaataatat tgaaaaagga 120 agagtatgag tattcaacat ttccgtgtcg cccttattcc cttttttgcg gcattttgcc 180 ttcctgtttt tgctcaccca gaaacgctgg tgaaagtaaa agatgctgaa gatcagttgg 240 gtgcacgagt gggttacatc gaactggatc tcaacagcgg taagatcctt gagagttttc 300 gccccgaaga acgttttcca atgatgagca cttttaaagt tctgctatgt ggcgcggtat 360 tatcccgtat tgacgccggg caagagcaac tcggtcgccg catacactat tctcagaatg 420 acttggttga gtactcacca gtcacagaaa agcatcttac ggatggcatg acagtaagag 480 aattatgcag tgctgccata accatgagtg ataacactgc ggccaactta cttctgacaa 540 cgatcggagg accgaaggag ctaaccgctt ttttgcacaa catgggggat catgtaactc 600 gccttgatcg ttgggaaccg gagctgaatg aagccatacc aaacgacgag cgtgacacca 660 cgatgcctgt agcaatggca acaacgttgc gcaaactatt aactggcgaa ctacttactc 720 tagcttcccg gcaacaatta atagactgga tggaggcgga taaagttgca ggaccacttc 780 tgcgctcggc ccttccggct ggctggttta ttgctgataa atctggagcc ggtgagcgtg 840 ggtctcgcgg tatcattgca gcactggggc cagatggtaa gccctcccgt atcgtagtta 900 tctacacgac ggggagtcag gcaactatgg atgaacgaaa tagacagatc gctgagatag 960 gtgcctcact gattaagcat tggtaactgt cagaccaagt ttactcatat atactttaga 1020 ttgatttaaa acttcatttt taatttaaaa ggatctaggt gaagatcctt tttgataatc 1080 tcatgaccaa aatcccttaa cgtgagtttt cgttccactg agcgtcagac cccgtagaaa 1140 agatcaaagg atcttcttga gatccttttt ttctgcgcgt aatctgctgc ttgcaaacaa 1200 aaaaaccacc gctaccagcg gtggtttgtt tgccggatca agagctacca actctttttc 1260 cgaaggtaac tggcttcagc agagcgcaga taccaaatac tgtccttcta gtgtagccgt 1320 agttaggcca ccacttcaag aactctgtag caccgcctac atacctcgct ctgctaatcc 1380 tgttaccagt ggctgctgcc agtggcgata agtcgtgtct taccgggttg gactcaagac 1440 gatagttacc ggataaggcg cagcggtcgg gctgaacggg gggttcgtgc acacagccca 1500 gcttggagcg aacgacctac accgaactga gatacctaca gcgtgagcta tgagaaagcg 1560 ccacgcttcc cgaagggaga aaggcggaca ggtatccggt aagcggcagg gtcggaacag 1620 gagagcgcac gagggagctt ccagggggaa acgcctggta tctttatagt cctgtcgggt 1680 ttcgccacct ctgacttgag cgtcgatttt tgtgatgctc gtcagggggg cggagcctat 1740 ggaaaaacgc cagcaacgcg gcctttttac ggttcctggc cttttgctgg ccttttgctc 1800 acatgttctt tcctgcgtta tcccctgatt ctgtggataa ccgtattacc gcctttgagt 1860 gagctgatac cgctcgccgc agccgaacga ccgagcgcag cgagtcagtg agcgaggaag 1920 cggagaagcg cccaatacgc aaaccgcctc tccccgcgcg ttggccgatt cattaatgca 1980 ggatctcgat cccgcgaaat taatacgact cactataggg agaccacaac ggtttccctc 2040 tagaaataat tttgtttaac tttaagaagg agatatacat atgaaacatc accaccatca 2100 ccattcggac tcagaagtca atcaagaagc taagccagag gtcaagccag aagtcaagcc 2160 tgagactcac atcaatttaa aggtgtccga tggatcttca gaaatcttct ttaagatcaa 2220 aaagaccact cctttaagaa ggctgatgga agcgttcgct aaaagacagg gtaaggaaat 2280 ggactcctta agattcttgt acgacggtat tagaattcaa gctgatcaga cccctgaaga 2340 tttggacatg gaggataacg atattattga ggctcacaga gaacagattg gtggcgccgc 2400 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2460 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2520 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2580 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2640 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2700 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2760 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2820 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2880 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgccgc 2940 tccagctgca cctgctccag cagcacctgc tgcaccagct ccggctgctc ctgctgcctg 3000 aagagcaagc ttgatccggc tgctaacaa gcccgaaagg aagctgagtt ggctgctgcc 3060 accgctgagc aataactagc ataacccctt ggggcctcta aacgggtctt gaggggtttt 3120 ttgctgaaag gaggaactat atccggatct ggcgtaatag cgaagaggcc cgcaccgatc 3180 gcccttccca acagttgcgc agcctgaatg gcgaatggga cgcgccctgt agcggcgcat 3240 taagcgcggc gggtgtggtg gttacgcgca gcgtgaccgc tacacttgcc agcgccctag 3300 cgcccgctcc tttcgctttc ttcccttcct ttctcgccac gttcgccggc tttccccgtc 3360 aagctctaaa tcgggggctc cctttagggt tccgatttag tgctttacgg cacctcgacc 3420 ccaaaaaact tgattagggt gatggttcac gtagtgggcc atcgccctga tagacggttt 3480 ttcgcccttt gacgttggag tccacgttct ttaatagtgg actcttgttc caaactggaa 3540 caacactcaa ccctatctcg gtctattctt ttgatttata agggattttg ccgatttcgg 3600 cctattggtt aaaaaatgag ctgatttaac aaaaatttaa cgcgaatttt aacaaaatat 3660 taacgcttac aatttaggtg 3680

(B) Analysis of the bacterially produced His(6)-SUMO-PA #1(200) fusion protein and its cleavage by 12% SDS-PAGE. The gel shows the SUMO-PAS #1(200) fusion protein extracted from E. coli and purified via immobilized metal affinity chromatography (IMAC) and size exclusion chromatography (SEC) before (lane 1) and after proteolytic cleavage with Ub1-specific protease 1 (SUMO protease) (lane 2) as described in Example 21. All samples were reduced with 2-mercaptoethanol. Sizes of protein markers (M), applied under reducing conditions, are indicated on the left margin. The His(6)-SUMO-PA #1(200) fusion protein appears as a single homogeneous band with an apparent molecular size of ca. 100 kDa. Thus, the apparent size for the His(6)-SUMO-PA #1(200) fusion protein observed in SDS-PAGE is significantly larger than the calculated mass of 28.3 kDa, which is due to the presence of the Pro/Ala polymer/polypeptide. After cleavage, the hydrophilic PA #1(200) polypeptide is not detectably stained by Coomassie blue; hence, only a small residual fraction of the fusion protein and the cleaved His(6)-SUMO protein are visible on the SDS polyacrylamide gel (lane 2). The His(6)-SUMO protein shows a homogeneous band with apparent molecular size of ca. 16 kDa (lane 2) which is well in agreement with its calculated molecular mass of 12.2 kDa.

FIG. 13: Conjugation of a biosynthetic Pro/Ala polymer/polypeptide with chemical compounds and/or drugs.

(A-D) Production of a fluorescein conjugate with a biosynthetic PA #1(200) polymer/polypeptide (SEQ ID NO: 61) monitored via analytical size exclusion chromatography (SEC). The panels show (from top to bottom) SEC runs of purified His(6)-SUMO-PA #1(200) (A), His(6)-SUMO-PA #1(200) after cleavage reaction in the presence of SUMO protease (B), the cleaved His(6)-SUMO-PA #1(200) batch after chemical coupling with a fluorescein NHS ester (C), and the fluorescein-PA #1(200) conjugate after IMAC purification (D). 250 μl of protein/polypeptide at a concentration of ca. 0.5 mg/ml was applied to a Superdex S200 10/300 GL column equilibrated with PBS on an Äkta purifier system. Absorption at 225 nm, 280 nm, and 494 nm was monitored using a UV-900 UV/VIS detector (GE Healthcare) and a prominent peak of each chromatogram was normalized to a value of 1. The arrow indicates the void volume of the column (7.3 ml).

(E-K) Characterization of free fluorescein, the biosynthetic PA #1(200) polymer/polypeptide, and its fluorescein conjugate via SEC and UV/VIS spectroscopy. The three chromatograms show (from top to bottom) purified PA #1(200) (E), the chemical compound fluorescein (F) and the purified fluorescein-PA #1(200) conjugate (G). The four UV/VIS spectra show the purified His(6)-SUMO-PA #1(200) fusion protein (H), the purified PA #1(200) polymer/polypeptide (I), free fluorescein (J), and the purified fluorescein-PA #1(200) conjugate (K) (all in PBS). The arrows indicate characteristic absorption bands/shoulders of SUMO (280 nm), PA #1(200) (225 nm), and fluorescein (494 nm).

(L) Calibration curve for the chromatograms from (A-G) using a Superdex S200 10/300 GL column. The logarithm of the molecular weight (MW) of marker proteins (aprotinin, 6.5 kDa; cytochrome C, 12.4 kDa; carbonic anhydrase, 29.0 kDa; bovine serum albumin, 66.3 kDa; alcohol dehydrogenase, 150 kDa; β-amylase, 200 kDa; apo-ferritin, 440 kDa) was plotted vs. their elution volumes (x) and fitted by a straight line. From the observed elution volumes of His(6)-SUMO-PA #1(200) (10.81 ml), PA #1(200) (11.51 ml), fluorescein-PA #1(200) (11.49 ml) and fluorescein (27.57 ml), their apparent molecular sizes were determined as follows. His(6)-SUMO-PA #1(200): 215.6 kDa, PA #1(200): 154.1 kDa (true mass: 16.1 kDa), fluorescein-PA #1(200): 155.6 kDa (true mass: 16.6 kDa); SUMO: 25.7 kDa (true mass: 12.2 kDa); fluorescein: 0.09 kDa (true mass: 0.33 kDa). These data show that fusion with the Pro/Ala polypeptide/polymer confers a much enlarged hydrodynamic volume to the conjugated drug compared with the unmodified compound.

(M) Characterization of the chemical conjugate between the biosynthetic PA #1(200) polypeptide/polymer and the steroid compound digoxigenin via Electro Spray Ionisation Mass Spectrometry (ESI-MS). A deconvoluted ESI-MS spectrum of digoxigenin-PA #1(200) reveals a mass of 16671.4 Da, which essentially coincides with the calculated mass for the digoxigenin-PA #1(200) conjugate (16670.6 Da).

FIG. 14: Illustration of chemical conjugates between the biosynthetic PA #1(200) polypeptide/polymer and small molecule drugs.

(A) Fluorescein coupled to the N-terminus of biosynthetic PA #1(200).

(B) Digoxigenin coupled to the N-terminus of biosynthetic PA #1(200).

EXAMPLES

The present invention is additionally described by way of the following illustrative non-limiting examples that provide a better understanding of the present invention and of its many advantages.

Unless otherwise indicated, established methods of recombinant gene technology were used as described, for example, in Sambrook (2001) loc. cit.

Example 1: Gene Synthesis for Pro/Ala Amino Acid Polymers/Polypeptides

As described herein above, amino acid repeats consisting of Pro and Ala residues are depicted herein as Pro/Ala or “PA”. Gene fragments encoding a repetitive polymer sequence comprising Pro and Ala (PA #1 which corresponds to SEQ ID NO: 1) were obtained by hybridisation of the two complementary oligodeoxynucleotides (SEQ ID NO: 17 and SEQ ID NO: 18) shown in FIG. 1, followed by concatamer formation in a directed manner via DNA ligation of their mutually compatible but non-palindromic sticky ends. Oligodeoxynucleotides were purchased from ThermoScientific (Ulm, Germany) and purified by preparative urea polyacrylamide gel electrophoresis. The nucleic acid sequences of the oligodesoxynucleotides are depicted in FIG. 1 (SEQ ID NOs 17 and 18 comprising an additional GCC codon for alanine, which becomes part of the following PA #1 sequence repeat upon ligation of the corresponding sticky ends. Enzymatic phosphorylation was performed by mixing 200 pmol of both oligodeoxynucleotides in 100 μl 50 mM Tris/HCl pH 7.6, 10 mM MgCl₂, 5 mM DTT, 1 mM ATP and incubation for 30 min at 37° C. in the presence of 10 u polynucleotide kinase (MBI Fermentas, St. Leon-Rot, Germany). After denaturation for 10 min at 80° C., the mixture was cooled to room temperature overnight to achieve hybridization. Then 50 μl of this solution was ligated by adding 1 u T4 DNA ligase (MBI Fermentas) and 10 μl 100 mM Tris/HCl pH 7.4, 50 mM MgCl₂, 20 mM DTT, 10 mM ATP, and in some cases 5 mM of each dATP, dCTP, dGTP, and dTTP, in a total volume of 100 μl and incubation for 55 min on ice. After 10 min heat inactivation at 70° C. the ligation products were separated by 1.5% (w/v) agarose gel electrophoresis in the presence of TAE buffer (40 mM Tris, 20 mM acetic acid, 1 mM EDTA). After staining with ethidium bromide the band corresponding to the assembled gene segment of 300 bp length was excised and isolated.

Example 2: Construction of pFab-PA #1(200) as Expression Vector for a Fab-PA #1 Fusion Protein

For cloning of a 10mer repeat of the synthetic gene fragment coding for the 20 amino acid sequence of PA #1 from Example 1 the plasmid vector pASK88-Fab-2×SapI (SEQ ID NO: 22), an expression plasmid for an Fab fragment (Schlapschy (2007) Protein Eng. Des. Sel. 20:273-284) harboring a nucleotide sequence with two SapI restriction sites in reverse complementary orientation at the 3-′end of the light chain (FIG. 2A), was employed. This vector, which is a derivative of pASK75 (Skerra, A. (1994) Gene 151:131-135), was cut with SapI, dephosphorylated with shrimp alkaline phosphatase (USB, Cleveland, Ohio), and ligated with a 300 bp cassette of the synthetic DNA fragment obtained from Example 1. The resulting intermediate plasmid pFab-PA #1(100) was again cut with SapI, dephosphorylated with shrimp alkaline phosphatase, and ligated with a 300 bp cassette of the synthetic DNA fragment obtained from Example 1 (as exemplified in FIG. 2B, however with only a PA #1(20) polymer/polypeptide cassette). The resulting plasmid was designated pFab-PA #1(200) (SEQ ID NO: 28) (FIG. 2C). It should be noted that on this plasmid the coding region for the 200 residue PA #1 sequence repeat was flanked by two SapI restriction, which enables precise excision and further subcloning of the entire sequence cassette, carrying 5′-GCC nucleotide overhangs.

After transformation of E. coli XL1-Blue (Bullock (1987) Biotechniques 5: 376-378), plasmid was prepared and the sequence of the cloned synthetic nucleic acid insert was confirmed by restriction analysis and double-stranded DNA sequencing (ABI-Prism™310 Genetic analyzer, Perkin-Elmer Applied Biosystems, Weiterstadt, Germany) using the BigDye™ terminator kit as well as oligodeoxynucleotide primers that enabled sequencing from both sides.

Example 3: Construction of pASK-PA #1(200)-IFNa2b as an Expression Vector for a PA #1(200)-IFNa2b Fusion Protein

For the construction of an expression plasmid encoding IFNa2b as fusion with a 200 residue PA #1 sequence repeat, PA #1(200), pASK-IFNa2b (SEQ ID NO: 32) (FIG. 2D) was cut with SapI, dephosphorylated with shrimp alkaline phosphatase, and ligated with the gene fragment encoding the 200 residue PA #1 polypeptide excised from the previously constructed plasmid pFab-PA #1(200) (Example 2) by restriction digest with SapI (as exemplified in FIG. 2E, however with only a PA #1(20) polymer/polypeptide cassette). After transformation of E. coli JM83 (Yanisch-Perron. (1985) Gene 33:103-119), plasmid was prepared and the presence of the correct insert was confirmed by restriction analysis. The resulting plasmid was designated pPA #1(200)-IFNa2b (SEQ ID NO: 37) (FIG. 2F).

Example 4: Bacterial Production and Purification of Fusion Proteins Between an Fab Fragment and a Genetically Encoded PA #1 Polymer/Polypeptide

The Fab fragment (calculated mass: 48.0 kDa) and the Fab-PA #1(200) fusion (calculated mass: 64.3 kDa) were produced at 22° C. in E. coli KS272 harboring the corresponding expression plasmids from Example 3, together with the folding helper plasmid pTUM4 (Schlapschy (2006) Protein Eng. Des. Sel. 19:385-390), using shaker flask cultures with 2 L LB medium containing 100 mg/l ampicillin and 30 mg/l chloramphenicol. Induction of recombinant gene expression was performed by addition of 0.4 mg anhydrotetracycline at OD₅₅₀=0.5 over night (typically resulting in OD₅₅₀ of ca. 1.0 at harvest). Periplasmic extraction in the presence of 500 mM sucrose, 1 mM EDTA, 100 mM Tris/HCl pH 8.0 containing 50 μg/ml lysozyme was performed as described elsewhere (Breustedt (2005) Biochim. Biophys. Acta 1764:161-173) and followed by purification by means of the His₆-tag using immobilized metal affinity chromatography (Skerra (1994) Gene 141: 79-84) with an imidazole gradient from 0 to 200 mM in 500 mM betaine, 50 mM Na-phosphate pH 7.5).

Homogeneous protein preparations were obtained for both recombinant Fab fragments (FIG. 3A) with yields of 0.2 mg L⁻¹ OD⁻¹ for the unfused Fab and 0.1 mg L⁻¹ OD⁻¹ for Fab-PA #1(200). SDS-PAGE was performed using a high molarity Tris buffer system (Fling (1986) Anal. Biochem. 155: 83-88). Protein concentrations were determined according to the absorption at 280 nm using calculated extinction coefficients (Gill (1989) Anal. Biochem. 182: 319-326) of 68290 M⁻¹ cm⁻¹ both for the unfused Fab and its PA #1 polymer fusion as the Pro/Ala polymer did not contribute to UV absorption because of its lack of aromatic amino acids.

Example 5: Bacterial Production and Purification of Fusion Proteins Between IFNa2b and a Genetically Encoded PA #1 Polymer/Polypeptide

IFNa2b (calculated mass: 20.9 kDa) and PA #1(200)-IFNa2b (calculated mass: 37.0 kDa) were produced at 22° C. in E. coli KS272 harboring the corresponding expression plasmids from Example 3, together with the folding helper plasmid pTUM4 (Schlapschy (2006) loc. cit.), using shaker flask cultures with 2 L LB medium containing 100 mg/l ampicillin and 30 mg/l chloramphenicol. Induction of recombinant gene expression was performed by addition of 0.4 mg anhydrotetracycline at OD₅₅₀=0.5 over night (typically resulting in OD₅₅₀ of ca. 1.0 at harvest). Periplasmic extraction in the presence of 500 mM sucrose, 1 mM EDTA, 100 mM Tris/HCl pH 8.0 containing 50 μg/ml lysozyme was performed as described elsewhere (Breustedt (2005) loc. cit.) and followed by purification via the Strep-tag II using streptavidin affinity chromatography (Schmidt (2007) Nat. Protoc. 2:1528-1535) in the presence of 150 mM NaCl, 1 mM EDTA, 100 mM Tris/HCl, pH 8.0.

Homogeneous protein preparations were obtained for both recombinant IFNa2b proteins (FIG. 3B) with yields of 0.15 mg L⁻¹ OD⁻¹ for IFNa2b and 0.1 mg L⁻¹ OD⁻¹ for PA #1(200)-IFNa2b. SDS-PAGE was performed using a high molarity Tris buffer system (Fling (1986) loc. cit.). Protein concentrations were determined according to the absorption at 280 nm using calculated extinction coefficients (Gill (1989) loc. cit.) of 23590 M⁻¹ cm⁻¹ both for the unfused IFNa2b and its PA #1 polymer fusion.

Example 6: Measurement of the Hydrodynamic Volume for the Recombinant Fusion Protein Between a Fab Fragment and a Genetically Encoded PA #1 Polymer of 200 Residues by Analytical Gel Filtration

Size exclusion chromatography (SEC) was carried out on a Superdex S200 HR 10/300 GL column (GE Healthcare Europe, Freiburg, Germany) at a flow rate of 1 ml/min using an Äkta Purifier 10 system (GE Healthcare) with PBS (115 mM NaCl, 4 mM KH₂PO₄, 16 mM Na₂HPO₄; pH 7.4) as running buffer. 250 μl samples of the purified Fab fragment and its 200 residue PA #1 fusion, obtained from the metal affinity affinity chromatography as described in Example 4, were individually applied at a concentration of 0.25 mg/ml in PBS. Both proteins eluted in a single homogenous peak as shown in FIG. 4A.

For column calibration (FIG. 4B), 250 μl of an appropriate mixture of the following globular proteins (Sigma, Deisenhofen, Germany) were applied in PBS at protein concentrations between 0.2 mg/ml and 0.5 mg/ml: cytochrome c, 12.4 kDa; carbonic anhydrase, 29.0 kDa; ovalbumin, 43.0 kDa; bovine serum albumin, 66.3 kDa; alcohol dehydrogenase, 150 kDa; β-amylase, 200 kDa; apo-ferritin, 440 kDa.

As result, the fusion protein with the 200 residue PA #1 polymer/polypeptide exhibited a significantly larger size than corresponding globular proteins with the same molecular weight. The apparent size increase for Fab-PA #1(200) was 7.4-fold compared with the unfused Fab fragment whereas the true mass was only larger by 1.3-fold. This observation clearly indicates a much increased hydrodynamic volume conferred to the biologically active Fab fragment by the Pro/Ala polypeptide segment according to this invention.

Example 7: Measurement of the Hydrodynamic Volume for the Recombinant Fusion Protein Between IFNa2b and a Genetically Encoded PA #1 Polymer of 200 Residues by Analytical Gel Filtration

Size exclusion chromatography was carried out with IFNa2b and PA #1(200)-IFNa2b on a Superdex S200 HR 10/300 GL column (GE Healthcare) at a flow rate of 1 ml/min using an Äkta Purifier 10 system (GE Healthcare) similarly as described in Example 6. Both proteins eluted in a single homogenous peak as shown in FIG. 4C.

As result, the fusion protein with the 200 residue PA #1 polymer/polypeptide exhibited a significantly larger size than corresponding globular proteins with the same molecular weight (FIG. 4D). The apparent size increase for PA #1(200)-IFNa2b was 10.2-fold compared with the unfused IFNa2b protein whereas the true mass was only larger by 1.8-fold. This observation clearly indicates a much increased hydrodynamic volume conferred to the biologically active interferon by the Pro/-Ala polymer/polypeptide according to this invention.

Example 8: Detection of Random Coil Conformation for the Biosynthetic PA #1 Polymer Fused to a Fab Fragment Via Circular Dichroism Spectroscopy

Secondary structure was analysed using a J-810 spectropolarimeter (Jasco, Groß-Umstadt, Germany) equipped with a quartz cuvette 106-QS (0.1 mm path length; Hellma, Müllheim, Germany). Spectra were recorded from 190 to 250 nm at room temperature by accumulating 16 runs (bandwidth 1 nm, scan speed 100 nm/min, response 4 s) using 3.12 to 15.4 μM protein solutions obtained from Example 4 in 50 mM K₂SO₄, 20 mM K-phosphate pH 7.5. After correction for solution blanks, spectra were smoothed using the instrument software, and the molar ellipticity Θ_(M) was calculated according to the equation:

$\Theta_{M} = \frac{\Theta_{obs}}{c \cdot d}$ whereby Θ_(obs) denotes the measured ellipticity, c the protein concentration [mol/l], d the path length of the quartz cuvette [cm]. The Θ_(M) values were plotted against the wavelength using Kaleidagraph (Synergy Software, Reading, Pa.).

The measured circular dichroism (CD) spectrum for the recombinant Fab was in accordance with the β-sheet dominated immunglobuline fold, whereas the spectrum for the Fab-PA #1(200) fusion protein revealed a significant contribution of random coil conformation (FIG. 5A). To analyze the spectroscopic contribution by the Pro/Ala polypeptide segment in greater detail the molar difference CD spectrum with respect to the unfused Fab fragment was calculated (FIG. 5B) by subtraction of the latter spectrum from the one for Fab-PA #1(200). As result, a strong minimum around 200 nm, which is characteristic of random coil conformation, was observed. Thus, the Pro/Ala sequence as part of the recombinant fusion protein appears to be present as a random coil polymer under physiological buffer conditions.

Example 9: Detection of Random Coil Conformation for the Genetically Encoded PA #1 Polymer Fused to IFNa2b Via Circular Dichroism Spectroscopy

Secondary structure was analysed by CD measurements for IFNa2b and PA #1(200)-IFNa2b (obtained from Example 5) as described in Example 8 using 3.6 to 38.7 μM protein solutions. The spectrum of PA #1(200)-IFNa2b revealed significant contributions of a-helical secondary structure, indicative of the known α-helix bundle fold of interferon, as well as of random coil conformation (FIG. 5C). To analyze the spectroscopic contributions by the Pro/Ala polymer fusion partner in greater detail the molar difference CD spectrum with respect to the unfused IFNa2b was calculated by subtraction of the two individual spectra (FIG. 5D). As result, a strong minimum around 200 nm characteristic of random coil conformation was observed. Thus, the Pro/Ala polypeptide segment as part of the recombinant fusion protein appears to be present as a random coil polymer under aqueous buffer conditions.

Example 10: Quantitative Analysis of the Secondary Structure of the Fab Fragment, of IFNa2b and of their 200 Residue PA #1 Polymer Fusions

The secondary structure content of the Fab fragment, Fab-PA #1(200), IFNa2b, and PA #1(200)-IFNa2b was individually quantified from the corresponding CD spectra measured in Examples 8 and 9 using the secondary structure deconvolution program CDNN ver. 2.1 (Böhm (1992) Protein Eng. 5:191-195) with a set of 33 base spectra for the deconvolution of complex CD spectra The results of this analysis are provided in the following Table:

Fab- Diff: PA#1 (100)- Diff: Fab PA#1(200) PA#1(200) IFNa2b IFNa2b PA#1(200) α-helix 9.5% 7.5%  2.1% 38.2% 31.0% 0.7% anti-parallel 40.4% 3.1%   0% 1.8% 0.2% 4.6% β-sheet parallel 6.9% 1.3%  0.3% 8.4% 0.7% 0.6% β-sheet β-turn 6.2% 50.4% 78.6% 19.2% 75.2% 69.7% random coil 37.2% 63.4% 94.8% 35.9% 64.4% 97.5% Σ total 100.2% 125.8% 175.8%  103.5% 171.4% 170.0% Σ β-turn and 43.4% 113.8% 173.4%  55.1% 139.6% 169.1% random coil

Compared with the predominantly β-sheet secondary structure content of the recombinant Fab fragment, which is in accordance with its known immunoglobulin fold (see Eigenbrot (1993) J. Mol. Biol. 229:969-995), the fraction of unstructured conformation (comprising random coil and β-turn) clearly increases if the PA #1 polymer is fused to the Fab fragment. The difference CD spectrum for the Pro/Ala polypeptide segment reveals a clear random coil conformation. Analysis of the secondary structure shows the presence of a high fraction of unstructured conformations (comprising random coil and β-turn) which nearly comprise 100% of the total secondary structure. Similarly, compared with the predominantly a-helical secondary structure content of the recombinant IFNa2b, which is in accordance with its known three-dimensional structure as an α-helix bundle protein (Radhakrishnan (1996) Structure 4:1453-1463), the fraction of unstructured conformation for the whole protein clearly increases if the PA #1 polymer is fused to IFNa2b. The difference CD spectrum for the Pro/Ala polypeptide segment reveals a clear random coil conformation. Analysis of the secondary structure shows the presence of a high fraction of unstructured conformations (comprising random coil and β-turn) which nearly comprise 100% of the total secondary structure.

Different results were obtained when a theoretical analysis of the PA #1 polymer sequence was performed using the Chou-Fasman algorithm (Chou and Fasman (1974) Biochemistry 13: 222-245). The results of this analysis are illustrated in FIG. 7. This algorithm predicts 100% α-helical secondary structure, which is in clear contrast with the experimental data. Thus, this algorithm is not useful to confidently predict unstructured conformation for an amino acid polymer according to the invention.

Example 11: Construction of pASK75-His6-PA #1(200)-hGH as an Expression Vector for a His6-PA #1(200)-hGH Fusion Protein

For the construction of an expression plasmid encoding hGH as fusion with a 200 residue PA #1 sequence repeat, PA #1(200), pASK75-His6-hGH (SEQ ID NO: 41) (FIG. 6A) was cut with SapI, dephosphorylated with shrimp alkaline phosphatase, and ligated with the gene fragment encoding the 200 residue PA #1 polypeptide excised from the previously constructed plasmid pFab-PA #1(200) (Example 2) by restriction digest with SapI (as exemplified in FIG. 6B, with only a PA #1(20) polymer/polypeptide cassette). After transformation of E. coli JM83 (Yanisch-Perron. (1985) loc. cit.), plasmid was prepared and the presence of the correct insert was confirmed by restriction analysis. The resulting plasmid was designated pASK75-His6-PA #1(200)-hGH (SEQ ID NO: 46) (FIG. 6C).

Example 12: Construction of an Expression Vector for the Secretory Production of Human Growth Hormone Fused with a 200 Residue PA #1 Polymer/Polypeptide in Chinese Hamster Ovary Cells

The vector pASK75-His6-PA #1(200)-hGH (SEQ ID NO: 46), a derivative of pASK75 (Skerra (1994) loc. cit.), allowing prokaryotic production of the hGH PA #1 fusion protein, was cut with NheI and HindIII. This fragment was purified via agarose gel electrophoresis and ligated with the correspondingly cut vector pCHO (SEQ ID NO: 50). After transformation of E. coli XL1-Blue (Bullock (1987) loc. cit.), plasmid was prepared and the correct insertion of the fragment was verified via restriction analysis. The resulting plasmid, which codes for the hGH signal peptide fused to the His₆ tag, a PA #1(200) polypeptide segment, and the human growth hormone (hGH), was designated pCHO-PA #1(200)-hGH SEQ ID NO: 48) and is depicted in FIG. 6D.

Example 13: Secretory Production of a Fusion Protein Between Human Growth Hormone (hGH) and the Genetically Encoded PA #1 Polymer in CHO Cells

CHO-K1 cells ATCC No. CCL-61 were cultured in Quantum 263 medium (PAA Laboratories, Colbe, Germany) in a 100 mm plastic dish until 50% confluency was reached. Cells were transfected with 8 μg pCHO-PA #1(200)-hGH (SEQ ID NO: 48) or, for control, pCHO-hGH (SEQ ID NO: 49), a similar plasmid encoding hGH without the PA #1(200) sequence, using the Nanofectin Kit (PAA Laboratories, Colbe, Germany). After 6 h, cell culture medium was exchanged by 7 ml OptiMEM®-I reduced serum medium (Invitrogen, Darmstadt, Germany) and cells were incubated at 37° C. in a humidified atmosphere with 5% CO₂. After two days, 20 μl of the cell culture supernatant was taken and diluted with 5 μl SDS-PAGE loading buffer containing β-mercaptoethanol. After 5 min heating at 95° C., 15 μl of each sample was subjected to 12% SDS-PAGE. Following electro-transfer onto a nitrocellulose membrane (Schleicher & Schuell, Dassel, Germany) by means of a semi-dry blotting apparatus, the membrane was washed 3 times for 15 min with 10 ml PBST (PBS containing 0.1% v/v Tween 20). The membrane was incubated with 10 ml of a 1:1000 dilution of anti human growth hormone antibody ab1956 conjugated with horse radish peroxidase (Abcam, Cambridge, UK). After incubation for 1 h and washing the membrane twice for 5 min with 20 ml PBST and twice for 5 min with PBS, the chromogenic reaction was performed in the presence of 15 ml of SIGMAFAST™ 3,3-diaminobenzidine solution (Sigma-Aldrich Chemie, Munich, Germany). The reaction was stopped by washing with water and air-drying of the membrane. The blot revealed signals for both recombinant protein samples (FIG. 6E), thus proving secretory production of the hGH fusion protein with the PA #1 polypeptide in CHO cells.

Example 14: Bacterial Production and Purification of Fusion Proteins Between hGH and a Genetically Encoded PA #1 Polymer/Polypeptide

Human growth hormone (hGH) (calculated mass: 23.4 kDa), PA #1(200)-hGH (calculated mass: 39.6 kDa), PA #1(400)-hGH (calculated mass: 55.8 kDa) and PA #1(600)-hGH (calculated mass: 72.0 kDa) were produced in E. coli KS272 harboring the corresponding expression plasmids from Example 11 or their derivatives with a double (encoding 400 residues) or triple (600 residues) PA #1 sequence cassette, respectively. Bacterial production was performed at 22° C. in shaker flask cultures with 2 L LB medium containing 2.5 g/L glucose, 0.5 g/L proline and 100 mg/l ampicillin. Induction of recombinant gene expression was performed by addition of 0.4 mg anhydrotetracycline at OD₅₅₀=0.5 for 3 h. Periplasmic extraction in the presence of 500 mM sucrose, 1 mM EDTA, 100 mM Tris/HCl pH 8.0 containing 50 μg/ml lysozyme was carried out as described elsewhere (Breustedt (2005) loc. cit.) and followed by purification via the His₆-tag using the HisTrap High Performance affinity column (GE Healthcare) with 40 mM Na-phosphate pH 7.5, 0.5 M NaCl as buffer. Proteins were eluted using an imidazole concentration gradient from 0 to 150 mM (dissolved in the running buffer and adjusted with HCl to pH 7.5) and further purified via size exclusion chromatography using a Superdex 200-HR10/30 column (GE Healthcare) equilibrated with PBS (115 mM NaCl, 4 mM KH₂PO₄, 16 mM Na₂HPO₄, pH 7.4).

After size exclusion chromatography homogeneous protein preparations were obtained for all recombinant hGH fusion proteins without signs of aggregation and with yields of 1 mg L⁻¹ OD⁻¹ for hGH, 0.3 mg L⁻¹ OD⁻¹ for PA #1(200)-hGH, 0.3 mg L⁻¹ OD⁻¹ for PA #1(400)-hGH and 0.2 mg L⁻¹ OD⁻¹ for PA #1(600)-hGH. SDS-PAGE was performed using a high molarity Tris buffer system (Fling (1986) loc. cit.). Protein concentrations were determined according to the absorption at 280 nm using calculated extinction coefficients (Gill (1989) loc. cit.) of 16050 M⁻¹ cm⁻¹ for the unfused hGH and all its PA #1 polypeptide fusions.

Example 15: Measurement of Binding Affinity of Human Growth Hormone and its PA #1 Polymer Fusions Towards the Extracellular Domain of Human Growth Hormone Receptor Using Surface Plasmon Resonance

The affinity of hGH and its PA #1 polypeptide fusions to a human growth hormone receptor Fc fusion protein (hGHR-Fc; R&D Systems) was determined via surface plasmon resonance (SPR) real time measurements on a Biacore 2000 system (GE Healthcare). First, 15 μl mouse anti-human IgG-Fc capture antibody (Jackson Immuno Research) at a concentration of 100 μg/ml in 10 mM Na-acetate pH 5.0 was immobilized to the surface of two flow channels of a CMDP chip (XanTec bioanalytics) using an amine coupling kit (GE Healthcare). This resulted in ca. 2700 response units (RU). After equilibration with PBS/T (PBS containing 0.05% (v/v) Tween 20) as flow buffer, one channel of the chip was charged with 2 μg/ml hGHR-Fc at a flow rate of 5 μl/min until an additional signal of ca. 300 RU was reached. Then, 75 μl of hGH or its PA #1 polypeptide fusions in PBS/T was injected at varying concentrations and the association and dissociation phases were measured under continuous buffer flow of 20 μl/min. For regeneration, three 6 μl pulses of 10 mM glycine/HCl pH 2.7 were applied. The sensograms were corrected by double subtraction of the corresponding signals measured for the channel without immobilized receptor and an averaged baseline determined from several buffer blank injections (Myszka (1999) Mol. Recognit. 12: 279-284). Kinetic data evaluation was performed by a global fit of the traces from at least seven different sample injections according to the 1:1 Langmuir binding model using BIAevaluation software version 3.1 (GE Healthcare). The values obtained from SPR measurements for the kinetic and derived equilibrium constants of the complexes between hGH or its PA #1 fusions and the human growth hormone receptor are summarized in the following Table:

hGH variant k_(on) [10⁵ M⁻¹ s⁻¹] k_(off) [10⁻⁶ s⁻¹] K_(D) [pM] hGH 10.2 10.6 10.4 PA#1(200)-hGH 4.75 9.18 19.3 PA#1(400)-hGH 3.26 14.0 42.9 PA#1(600)-hGH 3.29 12.5 38.0

These data show that the fusion of hGH with PA #1 polypeptides of different lengths does not significantly interfere with receptor binding. All hGH PA #1 polypeptide fusions retain receptor binding activity within a factor 5 compared with the recombinant hGH lacking a PA #1 polypeptide.

Example 16: Detection of Prolonged Plasma Half-Life In Vivo for the Recombinant Fusion Proteins Between a Fab Fragment and Genetically Encoded PA #1 Polymers

Adult BALB/c mice (SPF stock breeding; TU München, Freising, Germany) were intravenously injected according to the following Table:

Group A B D Test item Fab Fab- Fab- PA#1(200) PA#1(600) Administration route intravenous Dose [mg/kg b.w.] 5.0 5.0 5.0 Concentration [mg/ml] 1.0 1.0 1.0 Application volume [ml/kg b.w.] 5.0 No. of animals/group 9 9 9 No. of blood sampling time points 12 12 12 No. of animals/sampling time point 3 3 3 No. of blood samplings/animal 4/1 4/1 4/1

The total volume of intravenously administered test item was calculated according to the individual body weight (b.w.) recorded on the day of administration (e.g. an animal with 20 g body weight received 100 μl of 1 mg/ml test item). Blood sampling was performed according to the following Table:

Time points for blood sampling after injection Test item Subgroup 10 min 30 min 1 h 2 h 3 h 4 h 6 h 8 h 12 h 24 h 36 h 48 h Fab 1 x x x x Fab-PA#1(200) x x x x Fab-PA#1(600) x x x x 2 x x x x x x x x x x x x 3 x x x x x x x x x x x x

For each substance (Test item) altogether nine animals—divided into three subgroups 1-3 with each three animals—were injected, each providing four samples at different time points. Blood samples (approximately 50 μl) were taken from the tail vene and stored at 4° C. for 30 min. After centrifugation for 10 min at 10 000 g and 4° C. the supernatant (plasma) was immediately frozen and stored at −20° C.

For quantitative detection of the Fab fusion protein in an ELISA, the wells of a 96 well microtiter plate (Maxisorb, NUNC, Denmark) were coated overnight at 4° C. with 50 μl of a 10 μg/ml solution of recombinant Her2/ErbB2 ectodomain antigen in 50 mM NaHCO₃ pH 9.6. Then, the wells were blocked with 200 μl of 3% (w/v) BSA in PBS for 1 h and washed three times with PBS/T (PBS containing 0.1% (v/v) Tween 20). The plasma samples were applied in dilution series in PBS/T containing 0.5% (v/v) mouse plasma from an untreated animal and incubated for 1 h. The wells were then washed three times with PBS/T and incubated for 1 h with 50 μl of a 1:1000 diluted solution of an anti-human Cκ antibody alkaline phosphatase conjugate in PBS/T. After washing twice with PBS/T and twice with PBS the chromogenic reaction was started by adding 50 μl of 0.5 μg/ml p-nitrophenyl phosphate in 100 mM Tris/HCl pH 8.8, 100 mM NaCl, 5 mM MgCl₂ as substrate, and after 15 min at 25° C. the absorbance at 405 nm was measured. Concentrations of Fab, Fab-PA #1(200), and Fab-PA #1(600) in the plasma samples were quantified by comparison of the measured signals with standard curves which were determined for dilution series for the corresponding purified proteins at defined concentrations in PBS/T containing 0.5% (v/v) mouse plasma from untreated animals.

To estimate the plasma half-life of Fab, Fab-PA #1(200), and Fab-PA #1(600), the concentration values, c(t), were determined for each time point from the ELISA measurements and plotted against time post intravenous injection, t. These data were numerically fitted using KaleidaGraph software assuming a bi-exponential decay according to the equation

${c(t)} = {{c_{\alpha}e^{{- \ln}\; 2\;\frac{t}{\tau_{1/2}^{\alpha}}}} + {\left( {c_{0} - c_{\alpha}} \right)e^{{- \ln}\; 2\;\frac{t}{\tau_{1/2}^{\beta}}}}}$ whereby τ^(α) _(1/2) and τ^(β) _(1/2) are the half-life values of the distribution phase α and the elimination phase β, respectively. c₀ is the total blood concentration at time point zero while c_(α) is the concentration amplitude for the distribution phase.

FIG. 8 depicts the pharmacokinetics for the three test items in BALB/c mice. While the recombinant Fab shows a rapid blood clearance with an elimination half-life of just ca. 1.3 h, the Fab-PA #1(200) and Fab-PA #1(600) fusion proteins have a more than 3-fold and 29-fold extended half-life with corresponding values of ca. 4.1 h and 38.8 h, respectively. These data prove that the in vivo plasma half-life of a Fab fragment is significantly prolonged due to fusion with a Pro/Ala polymer/polypeptide, whereby the half-life becomes longer with increasing length of the amino acid polymer.

Example 17: Gene Synthesis for P1A1 and P1A3 Amino Acid Polymers/Polypeptides and Construction of pFab-P1A1(200) and pFab-P1A3(200) as Expression Vectors for Fab-P1A1(200) and Fab-P1A3(200) Fusion Proteins

Gene fragments encoding a repetitive polymer sequence comprising the Pro/Ala polypeptides/polymers P1A1 (SEQ ID NO: 51) and P1A3, also designated PA #3, (SEQ ID NO: 3) were obtained by hybridisation of pairs of complementary oligodeoxynucleotides, respectively, SEQ ID NO: 52 and SEQ ID NO: 53 for P1A1 and SEQ ID NO: 54 and SEQ ID NO: 55 for P1A3 as described in Example 1. pFab-P1A1(200) (Seq ID NO: 58) and pFab-P1A3(200) (Seq ID NO: 59) coding for Fab fragments with the corresponding Pro/Ala polymers/polypeptide segments of 200 residues at the C-terminus of the light chain (LC) (amino acid sequence of LC Fab-P1A1(200): SEQ ID NO: 56; amino acid sequence of LC Fab-P1A3(200): SEQ ID NO: 57) were constructed in an analogous manner to pFab-PA #1(200), which has been described in Example 2.

In the following SEQ ID NOs: 56, 57, 58 and 59 are also reproduced. However, these sequences are also comprised in the appended sequence listing which is a specific part of this disclosure and the description of the present invention.

SEQ ID NO: 56 Asp Ile Glu Leu Thr Gln Ser Pro Ser Ser Leu Ser Ala Ser Val Gly 1               5                   10                  15 Asp Arg Val Thr Ile Thr Cys Arg Ala Ser Gln Asp Val Asn Thr Ala             20                  25                  30 Val Ala Trp Tyr Gln Gln Lys Pro Gly Lys Ala Pro Lys Leu Leu Ile         35                  40                  45 Tyr Ser Ala Ser Phe Leu Tyr Ser Gly Val Pro Ser Arg Phe Ser Gly     50                  55                  60 Ser Arg Ser Gly Thr Asp Phe Thr Leu Thr Ile Ser Ser Leu Gln Pro 65                  70                  75                  80 Glu Asp Phe Ala Thr Tyr Tyr Cys Gln Gln His Tyr Thr Thr Pro Pro                 85                  90                  95 Thr Phe Gly Gln Gly Thr Lys Leu Glu Ile Lys Arg Thr Val Ala Ala             100                 105                 110 Pro Ser Val Phe Ile Phe Pro Pro Ser Asp Glu Gln Leu Lys Ser Gly         115                 120                 125 Thr Ala Ser Val Val Cys Leu Leu Asn Asn Phe Tyr Pro Arg Glu Ala     130                 135                 140 Lys Val Gln Trp Lys Val Asp Asn Ala Leu Gln Ser Gly Asn Ser Gln 145                 150                 155                 160 Glu Ser Val Thr Glu Gln Asp Ser Lys Asp Ser Thr Tyr Ser Leu Ser                 165                 170                 175 Ser Thr Leu Thr Leu Ser Lys Ala Asp Tyr Glu Lys His Lys Val Tyr             180                 185                 190 Ala Cys Glu Val Thr His Gln Gly Leu Ser Ser Pro Val Thr Lys Ser         195                 200                 205 Phe Asn Arg Gly Glu Cys Ser Ser Ala Pro Ala Pro Ala Pro Ala Pro     210                 215                 220 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro 225                 230                 235                 240 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro                 245                 250                 255 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro             260                 265                 270 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro         275                 280                 285 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro     290                 295                 300 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro 305                 310                 315                 320 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro                 325                 330                 335 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro             340                 345                 350 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro         355                 360                 365 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro     370                 375                 380 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro 385                 390                 395                 400 Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro Ala Pro                 405                 410                 415 Ala SEQ ID NO: 57 Asp Ile Glu Leu Thr Gln Ser Pro Ser Ser Leu Ser Ala Ser Val Gly 1               5                   10                  15 Asp Arg Val Thr Ile Thr Cys Arg Ala Ser Gln Asp Val Asn Thr Ala             20                  25                  30 Val Ala Trp Tyr Gln Gln Lys Pro Gly Lys Ala Pro Lys Leu Leu Ile         35                  40                  45 Tyr Ser Ala Ser Phe Leu Tyr Ser Gly Val Pro Ser Arg Phe Ser Gly     50                  55                  60 Ser Arg Ser Gly Thr Asp Phe Thr Leu Thr Ile Ser Ser Leu Gln Pro 65                  70                  75                  80 Glu Asp Phe Ala Thr Tyr Tyr Cys Gln Gln His Tyr Thr Thr Pro Pro                 85                  90                  95 Thr Phe Gly Gln Gly Thr Lys Leu Glu Ile Lys Arg Thr Val Ala Ala             100                 105                 110 Pro Ser Val Phe Ile Phe Pro Pro Ser Asp Glu Gln Leu Lys Ser Gly         115                 120                 125 Thr Ala Ser Val Val Cys Leu Leu Asn Asn Phe Tyr Pro Arg Glu Ala     130                 135                 140 Lys Val Gln Trp Lys Val Asp Asn Ala Leu Gln Ser Gly Asn Ser Gln 145                 150                 155                 160 Glu Ser Val Thr Glu Gln Asp Ser Lys Asp Ser Thr Tyr Ser Leu Ser                 165                 170                 175 Ser Thr Leu Thr Leu Ser Lys Ala Asp Tyr Glu Lys His Lys Val Tyr             180                 185                 190 Ala Cys Glu Val Thr His Gln Gly Leu Ser Ser Pro Val Thr Lys Ser         195                 200                 205 Phe Asn Arg Gly Glu Cys Ser Ser Ala Ala Ala Pro Ala Ala Ala Pro     210                 215                 220 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro 225                 230                 235                 240 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro                 245                 250                 255 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro             260                 265                 270 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro         275                 280                 285 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro     290                 295                 300 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro 305                 310                 315                 320 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro                 325                 330                 335 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro             340                 345                 350 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro         355                 360                 365 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro     370                 375                 380 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro 385                 390                 395                 400 Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro Ala Ala Ala Pro                 405                 410                 415 Ala SEQ ID NO: 58 acccgacacc atcgaatggc cagatgatta attcctaatt tttgttgaca ctctatcatt   60 gatagagtta ttttaccact ccctatcagt gatagagaaa agtgaaatga atagttcgac  120 aaaaatctag ataacgaggg caaaaaatga aaaagacagc tatcgcgatt gcagtggcac  180 tggctggttt cgctaccgta gcgcaggccg aagttaaact gcaggaatcc ggtggtggtc  240 tggttcagcc aggtggttcc ctgcggctct cgtgtgctgc ttccggtttc aacatcaaag  300 acacctacat ccactgggtt cgtcaggctc cgggtaaagg cctggaatgg gttgctcgta  360 tctacccgac caacggttac accaggtatg ccgattcagt taaaggtcgt ttcaccatct  420 cggccgacac ttccaaaaac accgcttacc tccagatgaa ctccctgcgt gctgaagaca  480 cagctgttta ttattgctcc cgttggggtg gtgacggttt ctacgctatg gactactggg  540 gtcagggtac cctggtcacc gtctcctcag cctccaccaa gggcccatcg gtcttccccc  600 tggcaccctc ctccaagagc acctctgggg gcacagcggc cctgggctgc ctggtcaagg  660 actacttccc cgaaccggtg acggtgtcgt ggaactcagg cgccctgacc agcggcgtgc  720 acaccttccc ggctgtccta cagtcctcag gactctactc cctcagcagc gtggtgactg  780 tgccctccag cagcttgggc acccagacct acatctgcaa cgttaatcac aaacccagca  840 acaccaaggt cgacaagaaa gttgagccca aatcttgcca tcaccaccat caccattaat  900 aaccatggag aaaataaagt gaaacaaagc actattgcac tggcactctt accgttactg  960 tttacccctg tgacaaaagc cgacatcgag ctcacccaat ccccgtcctc cctgtccgct 1020 tccgttggcg accgtgttac catcacgtgt agggcctcgc aagacgtaaa caccgccgta 1080 gcgtggtatc agcagaaacc cgggaaagct ccgaaactgc tgatctatag cgcttccttc 1140 ctgtattccg gagttccgag caggttcagt ggttcccgtt ccggtaccga cttcaccctg 1200 acgatatcct ccctccagcc ggaagacttc gctacctact actgtcaaca gcactacacc 1260 accccgccga ccttcggtca gggtaccaaa ctcgagatca aacggactgt ggctgcacca 1320 tctgtcttca tcttcccgcc atctgatgag cagttgaaat ctggaactgc ctctgttgtg 1380 tgcctgctga ataacttcta tcccagagag gccaaagtac agtggaaggt ggataacgcc 1440 ctccaatcgg gtaactccca ggagagtgtc acagagcagg acagcaagga cagcacctac 1500 agcctcagca gcaccctgac gctgagcaaa gcagactacg agaaacacaa agtctacgcc 1560 tgcgaagtca cccatcaggg cctgagttcg cccgtcacaa agagcttcaa ccgcggagag 1620 tgctcttctg cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1680 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1740 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1800 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1860 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1920 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 1980 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 2040 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 2100 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 2160 cctgcaccag cccctgctcc tgctccagca cctgcaccag cacctgctcc agcaccagct 2220 cctgcaccag cctgaagagc ttaagcttga cctgtgaagt gaaaaatggc gcacattgtg 2280 cgacattttt tttgtctgcc gtttaccgct actgcgtcac ggatctccac gcgccctgta 2340 gcggcgcatt aagcgcggcg ggtgtggtgg ttacgcgcag cgtgaccgct acacttgcca 2400 gcgccctagc gcccgctcct ttcgctttct tcccttcctt tctcgccacg ttcgccggct 2460 ttccccgtca agctctaaat cgggggctcc ctttagggtt ccgatttagt gctttacggc 2520 acctcgaccc caaaaaactt gattagggtg atggttcacg tagtgggcca tcgccctgat 2580 agacggtttt tcgccctttg acgttggagt ccacgttctt taatagtgga ctcttgttcc 2640 aaactggaac aacactcaac cctatctcgg tctattcttt tgatttataa gggattttgc 2700 cgatttcggc ctattggtta aaaaatgagc tgatttaaca aaaatttaac gcgaatttta 2760 acaaaatatt aacgtttaca atttcaggtg gcacttttcg gggaaatgtg cgcggaaccc 2820 ctatttgttt atttttctaa atacattcaa atatgtatcc gctcatgaga caataaccct 2880 gataaatgct tcaataatat tgaaaaagga agagtatgag tattcaacat ttccgtgtcg 2940 cccttattcc cttttttgcg gcattttgcc ttcctgtttt tgctcaccca gaaacgctgg 3000 tgaaagtaaa agatgctgaa gatcagttgg gtgcacgagt gggttacatc gaactggatc 3060 tcaacagcgg taagatcctt gagagttttc gccccgaaga acgttttcca atgatgagca 3120 cttttaaagt tctgctatgt ggcgcggtat tatcccgtat tgacgccggg caagagcaac 3180 tcggtcgccg catacactat tctcagaatg acttggttga gtactcacca gtcacagaaa 3240 agcatcttac ggatggcatg acagtaagag aattatgcag tgctgccata accatgagtg 3300 ataacactgc ggccaactta cttctgacaa cgatcggagg accgaaggag ctaaccgctt 3360 ttttgcacaa catgggggat catgtaactc gccttgatcg ttgggaaccg gagctgaatg 3420 aagccatacc aaacgacgag cgtgacacca cgatgcctgt agcaatggca acaacgttgc 3480 gcaaactatt aactggcgaa ctacttactc tagcttcccg gcaacaattg atagactgga 3540 tggaggcgga taaagttgca ggaccacttc tgcgctcggc ccttccggct ggctggttta 3600 ttgctgataa atctggagcc ggtgagcgtg gctctcgcgg tatcattgca gcactggggc 3660 cagatggtaa gccctcccgt atcgtagtta tctacacgac ggggagtcag gcaactatgg 3720 atgaacgaaa tagacagatc gctgagatag gtgcctcact gattaagcat tggtaggaat 3780 taatgatgtc tcgtttagat aaaagtaaag tgattaacag cgcattagag ctgcttaatg 3840 aggtcggaat cgaaggttta acaacccgta aactcgccca gaagctaggt gtagagcagc 3900 ctacattgta ttggcatgta aaaaataagc gggctttgct cgacgcctta gccattgaga 3960 tgttagatag gcaccatact cacttttgcc ctttagaagg ggaaagctgg caagattttt 4020 tacgtaataa cgctaaaagt tttagatgtg ctttactaag tcatcgcgat ggagcaaaag 4080 tacatttagg tacacggcct acagaaaaac agtatgaaac tctcgaaaat caattagcct 4140 ttttatgcca acaaggtttt tcactagaga atgcattata tgcactcagc gcagtggggc 4200 attttacttt aggttgcgta ttggaagatc aagagcatca agtcgctaaa gaagaaaggg 4260 aaacacctac tactgatagt atgccgccat tattacgaca agctatcgaa ttatttgatc 4320 accaaggtgc agagccagcc ttcttattcg gccttgaatt gatcatatgc ggattagaaa 4380 aacaacttaa atgtgaaagt gggtcttaaa agcagcataa cctttttccg tgatggtaac 4440 ttcactagtt taaaaggatc taggtgaaga tcctttttga taatctcatg accaaaatcc 4500 cttaacgtga gttttcgttc cactgagcgt cagaccccgt agaaaagatc aaaggatctt 4560 cttgagatcc tttttttctg cgcgtaatct gctgcttgca aacaaaaaaa ccaccgctac 4620 cagcggtggt ttgtttgccg gatcaagagc taccaactct ttttccgaag gtaactggct 4680 tcagcagagc gcagatacca aatactgtcc ttctagtgta gccgtagtta ggccaccact 4740 tcaagaactc tgtagcaccg cctacatacc tcgctctgct aatcctgtta ccagtggctg 4800 ctgccagtgg cgataagtcg tgtcttaccg ggttggactc aagacgatag ttaccggata 4860 aggcgcagcg gtcgggctga acggggggtt cgtgcacaca gcccagcttg gagcgaacga 4920 cctacaccga actgagatac ctacagcgtg agctatgaga aagcgccacg cttcccgaag 4980 ggagaaaggc ggacaggtat ccggtaagcg gcagggtcgg aacaggagag cgcacgaggg 5040 agcttccagg gggaaacgcc tggtatcttt atagtcctgt cgggtttcgc cacctctgac 5100 ttgagcgtcg atttttgtga tgctcgtcag gggggcggag cctatggaaa aacgccagca 5160 acgcggcctt tttacggttc ctggcctttt gctggccttt tgctcacatg            5210 SEQ ID NO: 59 acccgacacc atcgaatggc cagatgatta attcctaatt tttgttgaca ctctatcatt   60 gatagagtta ttttaccact ccctatcagt gatagagaaa agtgaaatga atagttcgac  120 aaaaatctag ataacgaggg caaaaaatga aaaagacagc tatcgcgatt gcagtggcac  180 tggctggttt cgctaccgta gcgcaggccg aagttaaact gcaggaatcc ggtggtggtc  240 tggttcagcc aggtggttcc ctgcggctct cgtgtgctgc ttccggtttc aacatcaaag  300 acacctacat ccactgggtt cgtcaggctc cgggtaaagg cctggaatgg gttgctcgta  360 tctacccgac caacggttac accaggtatg ccgattcagt taaaggtcgt ttcaccatct  420 cggccgacac ttccaaaaac accgcttacc tccagatgaa ctccctgcgt gctgaagaca  480 cagctgttta ttattgctcc cgttggggtg gtgacggttt ctacgctatg gactactggg  540 gtcagggtac cctggtcacc gtctcctcag cctccaccaa gggcccatcg gtcttccccc  600 tggcaccctc ctccaagagc acctctgggg gcacagcggc cctgggctgc ctggtcaagg  660 actacttccc cgaaccggtg acggtgtcgt ggaactcagg cgccctgacc agcggcgtgc  720 acaccttccc ggctgtccta cagtcctcag gactctactc cctcagcagc gtggtgactg  780 tgccctccag cagcttgggc acccagacct acatctgcaa cgttaatcac aaacccagca  840 acaccaaggt cgacaagaaa gttgagccca aatcttgcca tcaccaccat caccattaat  900 aaccatggag aaaataaagt gaaacaaagc actattgcac tggcactctt accgttactg  960 tttacccctg tgacaaaagc cgacatcgag ctcacccaat ccccgtcctc cctgtccgct 1020 tccgttggcg accgtgttac catcacgtgt agggcctcgc aagacgtaaa caccgccgta 1080 gcgtggtatc agcagaaacc cgggaaagct ccgaaactgc tgatctatag cgcttccttc 1140 ctgtattccg gagttccgag caggttcagt ggttcccgtt ccggtaccga cttcaccctg 1200 acgatatcct ccctccagcc ggaagacttc gctacctact actgtcaaca gcactacacc 1260 accccgccga ccttcggtca gggtaccaaa ctcgagatca aacggactgt ggctgcacca 1320 tctgtcttca tcttcccgcc atctgatgag cagttgaaat ctggaactgc ctctgttgtg 1380 tgcctgctga ataacttcta tcccagagag gccaaagtac agtggaaggt ggataacgcc 1440 ctccaatcgg gtaactccca ggagagtgtc acagagcagg acagcaagga cagcacctac 1500 agcctcagca gcaccctgac gctgagcaaa gcagactacg agaaacacaa agtctacgcc 1560 tgcgaagtca cccatcaggg cctgagttcg cccgtcacaa agagcttcaa ccgcggagag 1620 tgctcttctg ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1680 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1740 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1800 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1860 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1920 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 1980 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 2040 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 2100 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 2160 gcagctccag ccgctgcacc tgctgcagca cctgctgcag ctccagcagc tgctcctgca 2220 gcagctccag cctgaagagc ttaagcttga cctgtgaagt gaaaaatggc gcacattgtg 2280 cgacattttt tttgtctgcc gtttaccgct actgcgtcac ggatctccac gcgccctgta 2340 gcggcgcatt aagcgcggcg ggtgtggtgg ttacgcgcag cgtgaccgct acacttgcca 2400 gcgccctagc gcccgctcct ttcgctttct tcccttcctt tctcgccacg ttcgccggct 2460 ttccccgtca agctctaaat cgggggctcc ctttagggtt ccgatttagt gctttacggc 2520 acctcgaccc caaaaaactt gattagggtg atggttcacg tagtgggcca tcgccctgat 2580 agacggtttt tcgccctttg acgttggagt ccacgttctt taatagtgga ctcttgttcc 2640 aaactggaac aacactcaac cctatctcgg tctattcttt tgatttataa gggattttgc 2700 cgatttcggc ctattggtta aaaaatgagc tgatttaaca aaaatttaac gcgaatttta 2760 acaaaatatt aacgtttaca atttcaggtg gcacttttcg gggaaatgtg cgcggaaccc 2820 ctatttgttt atttttctaa atacattcaa atatgtatcc gctcatgaga caataaccct 2880 gataaatgct tcaataatat tgaaaaagga agagtatgag tattcaacat ttccgtgtcg 2940 cccttattcc cttttttgcg gcattttgcc ttcctgtttt tgctcaccca gaaacgctgg 3000 tgaaagtaaa agatgctgaa gatcagttgg gtgcacgagt gggttacatc gaactggatc 3060 tcaacagcgg taagatcctt gagagttttc gccccgaaga acgttttcca atgatgagca 3120 cttttaaagt tctgctatgt ggcgcggtat tatcccgtat tgacgccggg caagagcaac 3180 tcggtcgccg catacactat tctcagaatg acttggttga gtactcacca gtcacagaaa 3240 agcatcttac ggatggcatg acagtaagag aattatgcag tgctgccata accatgagtg 3300 ataacactgc ggccaactta cttctgacaa cgatcggagg accgaaggag ctaaccgctt 3360 ttttgcacaa catgggggat catgtaactc gccttgatcg ttgggaaccg gagctgaatg 3420 aagccatacc aaacgacgag cgtgacacca cgatgcctgt agcaatggca acaacgttgc 3480 gcaaactatt aactggcgaa ctacttactc tagcttcccg gcaacaattg atagactgga 3540 tggaggcgga taaagttgca ggaccacttc tgcgctcggc ccttccggct ggctggttta 3600 ttgctgataa atctggagcc ggtgagcgtg gctctcgcgg tatcattgca gcactggggc 3660 cagatggtaa gccctcccgt atcgtagtta tctacacgac ggggagtcag gcaactatgg 3720 atgaacgaaa tagacagatc gctgagatag gtgcctcact gattaagcat tggtaggaat 3780 taatgatgtc tcgtttagat aaaagtaaag tgattaacag cgcattagag ctgcttaatg 3840 aggtcggaat cgaaggttta acaacccgta aactcgccca gaagctaggt gtagagcagc 3900 ctacattgta ttggcatgta aaaaataagc gggctttgct cgacgcctta gccattgaga 3960 tgttagatag gcaccatact cacttttgcc ctttagaagg ggaaagctgg caagattttt 4020 tacgtaataa cgctaaaagt tttagatgtg ctttactaag tcatcgcgat ggagcaaaag 4080 tacatttagg tacacggcct acagaaaaac agtatgaaac tctcgaaaat caattagcct 4140 ttttatgcca acaaggtttt tcactagaga atgcattata tgcactcagc gcagtggggc 4200 attttacttt aggttgcgta ttggaagatc aagagcatca agtcgctaaa gaagaaaggg 4260 aaacacctac tactgatagt atgccgccat tattacgaca agctatcgaa ttatttgatc 4320 accaaggtgc agagccagcc ttcttattcg gccttgaatt gatcatatgc ggattagaaa 4380 aacaacttaa atgtgaaagt gggtcttaaa agcagcataa cctttttccg tgatggtaac 4440 ttcactagtt taaaaggatc taggtgaaga tcctttttga taatctcatg accaaaatcc 4500 cttaacgtga gttttcgttc cactgagcgt cagaccccgt agaaaagatc aaaggatctt 4560 cttgagatcc tttttttctg cgcgtaatct gctgcttgca aacaaaaaaa ccaccgctac 4620 cagcggtggt ttgtttgccg gatcaagagc taccaactct ttttccgaag gtaactggct 4680 tcagcagagc gcagatacca aatactgtcc ttctagtgta gccgtagtta ggccaccact 4740 tcaagaactc tgtagcaccg cctacatacc tcgctctgct aatcctgtta ccagtggctg 4800 ctgccagtgg cgataagtcg tgtcttaccg ggttggactc aagacgatag ttaccggata 4860 aggcgcagcg gtcgggctga acggggggtt cgtgcacaca gcccagcttg gagcgaacga 4920 cctacaccga actgagatac ctacagcgtg agctatgaga aagcgccacg cttcccgaag 4980 ggagaaaggc ggacaggtat ccggtaagcg gcagggtcgg aacaggagag cgcacgaggg 5040 agcttccagg gggaaacgcc tggtatcttt atagtcctgt cgggtttcgc cacctctgac 5100 ttgagcgtcg atttttgtga tgctcgtcag gggggcggag cctatggaaa aacgccagca 5160 acgcggcctt tttacggttc ctggcctttt gctggccttt tgctcacatg            5210

Example 18: Measurement of the Hydrodynamic Volume for the Recombinant Fusion Protein Between a Fab Fragment and a Genetically Encoded P1A1 or P1A3 Polypeptide/Polymer by Analytical Gel Filtration

SEC was carried out on a Superdex S200 HR 10/300 GL column (GE Healthcare Europe, Freiburg, Germany) at a flow rate of 1 ml/min using an Äkta Purifier 10 system (GE Healthcare) with PBS as running buffer. 250 μl samples of the Fab-P1A1(200) and Fab-P1A3(200) fusion proteins, which were similarly produced and purified (FIG. 9) as described for Fab-PA #1(200) in Example 4, were individually applied at a concentration of 0.25 mg/ml in PBS. Both proteins eluted in a single homogenous peak as shown in FIG. 10.

As result, the fusion proteins with the 200 residue P1A1 or P1A3 polymers/polypeptides exhibited significantly larger sizes than the corresponding unfused Fab fragment. The apparent size increase for Fab-P1A1(200) and Fab-P1A3(200) was 5.8-fold and 5.2-fold, respectively, compared with the Fab fragment (cf. FIG. 4B) whereas the true mass was only larger by 1.4-fold and 1.3-fold. This observation clearly indicates a much increased hydrodynamic volume conferred to the biologically active Fab fragment by the biosynthetic P1A1 and P1A3 polypeptide segments according to this invention.

Example 19: Detection of Random Coil Conformation for the Biosynthetic P1A1 and P1A3 Polymers/Polypeptides Fused to a Fab Fragment Via Circular Dichroism (CD) Spectroscopy

CD spectra for Fab-P1A1(200) and Fab-P1A3(200) were recorded as described in Example 8 using 4.2 and 6.5 μM protein solutions, respectively, prepared similarly as described in Example 4 using 50 mM K₂SO₄, 20 mM K-phosphate pH 7.5 as buffer.

The spectra for the Fab-P1A1(200) and Fab-P1A3(200) fusion proteins revealed a significant fraction of random coil conformation (FIG. 11A). To analyze the spectroscopic contribution by the Pro/Ala polypeptide segment in greater detail the molar difference CD spectrum with respect to the unfused Fab fragment (see Example 8) was calculated (FIG. 11B) by subtracting the latter spectrum from the one for Fab-P1A1(200) and Fab-P1A3(200), respectively, after normalization to the same molar concentration. As result, a strong minimum at a wavelength of approximately 200 nm, which is characteristic of random coil conformation, was observed. Thus, the P1A1 and the P1A3 sequences as part of the recombinant fusion protein appear to be present in random coil conformation under physiological buffer conditions.

Example 20: Construction of pSUMO-PA #1(200) as Expression Vector for a His(6)-SUMO-PA #1(200) Fusion Protein

For the construction of an expression plasmid encoding a six-residue His-tag and the small ubiquitin-like modifier (SUMO) protein (Panavas (2009) Methods Mol. Biol. 497: 303-17) fused to a 200 residue PA #1 sequence repeat, the SUMO protein) from Saccharomyces cerevisiae [also known as Smt3p; Uniprot: Q12306] was amplified via polymerase chain reaction (PCR) from a cloned cDNA. The 5′-primer introduced an NdeI restriction site, containing a Met start codon (ATG) and an additional Lys codon, as well as the His6-tag encoding sequence while the 3′-primer introduced a HindIII and SapI restriction site into the PCR product. The resulting DNA fragment was digested with NdeI and HindIII and ligated with a correspondingly digested derivative of the plasmid pSA1 (Schmidt (1994) J. Chromatogr. 676: 337-345), wherein the SapI restriction site had been eliminated by silent mutation. The resulting plasmid was cut with SapI, dephosphorylated with shrimp alkaline phosphatase, and ligated with the gene fragment encoding the 200 residue PA #1 polypeptide segment excised from the plasmid pFab-PA #1(200) (described in Example 2) by restriction digest with SapI (in an analogous way as exemplified in FIG. 2E). The resulting plasmid was designated pSUMO-PA #1(200) (SEQ ID NO: 60) and is depicted in FIG. 12A.

Example 21: Bacterial Expression and Isolation of a Genetically Encoded PA #1(200) Polymer/Polypeptide

The PA #1(200) polypeptide (calculated mass: 16.1 kDa) was initially produced as fusion protein with the small ubiquitin-like modifier (SUMO) protein (calculated mass: 12.2 kDa) in the cytoplasm of E. coli BLR(DE3) (NEB, Ipswich, Mass., USA) harboring the expression plasmid pSUMO-PA #1(200) (described in Example 21) together with the plasmid pLysE (Studier (1991) J. Mol. Biol. 219: 37-44), which suppresses the the T7 promoter. Bacterial production was performed at 30° C. in shake flask cultures with 2 L LB medium containing 2.5 g/L D-glucose, 0.5 g/L L-proline, 100 mg/l ampicillin, and 30 mg/l chloramphenicol. Recombinant gene expression was induced by addition of isopropyl-β-D-thiogalactopyranoside (IPTG) to a final concentration of 0.5 mM. Bacteria were harvested 3 h after induction, resuspended in 100 mM NaCl, 40 mM Na-phosphate pH 7.5 and lysed using a French pressure cell (Thermo Scientific, Waltham, Mass., USA). After centrifugation (15 min, 15000 g) of the lysate no inclusion bodies were observed.

The supernatant containing the soluble fusion protein was incubated at 70° C. for 15 min and centrifuged (15 min, 15000 g) to remove thermally unstable host cell proteins. The His(6)-SUMO-PA #1(200) fusion protein was purified from the supernatant via IMAC (Skerra (1994) Gene 141: 79-84) using a 12 ml Ni₂ ⁺ charged HisTrap high performance column (GE Healthcare) connected to an Äkta purifier system (GE Healthcare) and eluted with an imidazole gradient from 0 to 150 mM in 500 mM NaCl, 40 mM Na-phosphate pH 7.5. After a subsequent preparative SEC step a homogeneous preparation of the His(6)-SUMO-PA #1(200) fusion protein (FIG. 12B) with a yield of approximately 5 mg per 1 L bacterial culture with OD550=1 was obtained. Protein concentration was determined according to the absorption at 280 nm using a calculated extinction coefficient (Gill (1989) loc. cit) of 1280 M⁻¹ cm⁻¹ for the His(6)-SUMO-PA #1(200) polypeptide fusion. Note that the PA #1(200) polypeptide segment does not contribute to the absorption at 280 nm due to its lack of aromatic or sulfur-containing amino acid side chains.

The biosynthetic PA #1(200) polypeptide was liberated from the fusion protein by site specific proteolytic cleavage (downstream of a Gly-Gly motif preceding the Pro/Ala polypeptide segment) with 2 U/mg Ub1-specific protease 1 from Saccharomyces cerevisiae (Invitrogen, Carlsbad, Calif., USA) for 1 h at 30° C. in cleavage buffer (0.2 w/v % Igepal, 1 mM DTT, 150 mM NaCl, 50 mM Tris-HCl pH 8.0). The cleavage process was checked by SDS-PAGE (FIG. 12B) using a high molarity Tris buffer system (Fling (1986) Anal. Biochem. 155: 83-88). In order to remove the cleaved His(6)-SUMO protein, residual uncleaved fusion protein, and also the SUMO protease, all carrying the His₆-tag, the reaction mixture was subjected to another IMAC using a 5 ml Ni₂ ⁺ charged HisTrap high performance column (GE Healthcare) and 500 M NaCl, 20 mM phosphate, pH 7.5 as running buffer. This time the flow-through contained the pure biosynthetic PA #1(200) polypeptide (FIG. 13 E). Note that the biosynthetic PA #1(200) polypeptide/polymer (SEQ ID NO: 61) prepared in this manner comprises altogether 201 amino acid residues, which arise from the encoded combined gene product of 10 ligated double-stranded oligodeoxynucleotide building blocks, each encoding 20 amino acid residues, as shown in FIG. 1, and an additional Ala residue encoded by the triplet DNA overhang of the downstream SapI restriction site that was used for cloning.

Example 22: Preparation and Characterization of Small Molecule/Drug Conjugates with PA #1(200)

The unpurified proteolytic cleavage reaction mixture of the His(6)-SUMO-PA #1(200) fusion protein from Example 21 was twice dialysed at 4° C. against 50 mM NaHCO₃ pH 8.3 and incubated at room temperature for 1 h after mixing with a 10-fold molar excess of a solution of 6-[fluorescein-5(6)-carboxamido] hexanoic acid N-hydroxysuccinimide ester (Fluorescein-NHS ester; Sigma-Aldrich) in dry dimethylformamide (DMF). To this end, 200 μl of a 2.5 mg/ml solution of the His(6)-SUMO-PA #1(200) cleavage mixture was added to 17.6 μl of a 10 mM solution of Fluorescein-NHS ester dissolved in DMF. The resulting mixture was incubated at room temperature for 1 h and applied to IMAC as described in Example 21 to remove the cleaved His(6)-SUMO protein, residual uncleaved fusion protein, and the SUMO protease and further purified by preparative SEC on a Superdex S200 10/300 GL column equilibrated with PBS at a flow rate of 0.5 ml/min.

Samples from the different steps were then analysed via analytical SEC on a Superdex S200 10/300 GL column equilibrated with PBS at a flow rate of 0.5 ml/min. The SUMO protein was detected via its aromatic side chains at 280 nm and the peptide bonds, including those of the Pro/Ala polypeptide or polypeptide segment, were detected at 225 nm while fluorescein was detected at 494 nm (FIG. 13 A-G). For comparison, UV/VIS spectra of a solution of free fluorescein (Sigma-Aldrich) and of fractions from each distinct peak detected in the SEC were measured using a Lambda 9 instrument (Perkin Elmer, Waltham, Mass., USA) (FIG. 13 H-K). For size calibration of the chromatography column (FIG. 13 L), 250 μl of an appropriate mixture of the following globular proteins (Sigma-Aldrich) were applied in PBS at concentrations between 0.2 and 0.5 mg/ml: aprotinin, 6.5 kDa; cytochrome c, 12.4 kDa; carbonic anhydrase, 29.0 kDa; bovine serum albumin, 66.3 kDa; alcohol dehydrogenase, 150 kDa; β-amylase, 200 kDa; apo-ferritin, 440 kDa.

As result, after coupling of the biosynthetic PA #1(200) polypeptide/polymer with Fluorescein-NHS ester a macromolecular conjugate was isolated via IMAC and SEC that essentially exhibits the size properties of the PA #1(200) polypeptide/polymer and the spectroscopic signature of the small molecule, i.e. the fluorescein group. This demonstrates that the small molecule was successfully coupled to the biosynthetic Pro/Ala polypeptide/polymer, which according to this invention dramatically increases the hydrodynamic volume of the conjugated small molecule drug or compound.

To prepare a similar conjugate between the biosynthetic Pro/Ala polypeptide/polymer and the plant steroid digoxigenin, 0.1 mg of the purified PA #1(200) polypeptide from Example 21 was dialysed against 50 mM NaHCO₃ pH 8.3 as described above. The concentration of purified PA #1(200) polypeptide was determined according to the absorption at 205 nm (Gill (1989) loc. cit). The PA #1(200) polypeptide was coupled with a 10-fold molar excess of digoxigenin-3-O-methylcarbonyl-ε-aminocaproic acid NHS ester (DIG-NHS ester; Roche Diagnostics, Mannheim, Germany). For this purpose, 100 μl of a 1 mg/ml solution of the purified PA #1(200) polypeptide in 50 mM NaHCO₃ pH 8.3 was added to 2 μl of a 30 mM solution of DIG-NETS ester dissolved in dry DMF and the reaction mix was incubated for 1 h at room temperature. The resulting solution of the conjugate was purified using a Zeba™ spin desalting column with a cutoff of 7 kDa (Thermo Scientific), twice dialysed against 10 mM ammonium acetate buffer pH 6.8 and analysed via ESI mass spectrometry on a Q-Tof Ultima instrument (Waters, Eschbronn, Germany) using the positive ion mode. As result, the spectrum of the Digoxigenin-PA #1(200) conjugate revealed a mass of 16671.4 Da, which essentially coincides with the calculated mass of 16670.6 Da (FIG. 13M). This clearly demonstrates that a biosynthetic Pro/Ala polypeptide/polymer, in particular PA #1(200), can be efficiently conjugated with a small molecule drug.

The present invention relates to and refers to the following exemplified sequences, whereby the appended sequence listing is presented as part of the description and is, accordingly a part of this specification.

SEQ ID NO: 1 shows the amino acid sequence of PA #1.

SEQ ID NO: 2 shows the amino acid sequence of PA #2.

SEQ ID NO: 3 shows the amino acid sequence of PA #3.

SEQ ID NO: 4 shows the amino acid sequence of PA #4.

SEQ ID NO: 5 shows the amino acid sequence of PA #5.

SEQ ID NO: 6 shows the amino acid sequence of PA #6.

SEQ ID NO: 7 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1

SEQ ID NO: 8 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 9 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 10 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 11 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 12 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 13 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 14 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 15 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 16 shows an amino acid sequence of a circular permutated version of SEQ ID NO: 1.

SEQ ID NO: 17 shows a nucleic acid sequence of the upper/coding strand oligodeoxynucleotide used for the generation of building block PA #1.

SEQ ID NO: 18 shows a nucleic acid sequence of lower/non-coding strand oligodeoxynucleotide used for the generation of the building block for PA #1.

SEQ ID NO: 19 shows a nucleic acid sequence stretch (upper/coding strand) around the C-terminus of the immunoglobulin light chain of an antibody Fab fragment as encoded on pASK88-Fab-2×SapI.

SEQ ID NO: 20 shows a nucleic acid sequence stretch (lower/non-coding strand) around the C-terminus of the immunoglobulin light chain of an antibody Fab fragment as encoded on pASK88-Fab-2×SapI.

SEQ ID NO: 21 shows an amino acid sequence of the C-terminus of the light chain of the Fab fragment as encoded on pASK88-Fab-2×SapI.

SEQ ID NO: 22 shows the nucleic acid sequence of pASK88-Fab-2×SapI.

SEQ ID NO: 23 shows a nucleic acid sequence stretch (upper/coding strand) encoding amino acid sequence of the C-terminus of the Fab light chain after insertion of one PA #1(20) polymer.

SEQ ID NO: 24 shows a nucleic acid sequence (lower/non-coding strand) for an amino acid stretch of the C-terminus of an Fab light chain after insertion of one PA #1(20) polymer.

SEQ ID NO: 25 shows an amino acid sequence stretch of the C-terminus of an Fab light chain after insertion of one PA #1(20) polymer.

SEQ ID NO: 26 shows the amino acid sequence of the Fab heavy chain as encoded on pFab-PA #1(200).

SEQ ID NO: 27 shows the amino acid sequence of the Fab light chain fused with the PA #1(200) polymer as encoded on pFab-PA #1(200).

SEQ ID NO: 28 shows the nucleic acid sequence of pFab-PA #1(200).

SEQ ID NO: 29 shows the nucleic acid sequence (upper/coding strand) encoding the amino acid sequence of the N-terminus of INFa2b and Strep-tag II (only the last two amino acids).

SEQ ID NO: 30 shows a nucleic acid sequence (lower/non-coding strand) encoding amino acid sequence of the N-terminus of INFa2b and Strep-tag II (only the last two amino acids).

SEQ ID NO: 31 shows the amino acid sequence of the C-terminus of Strep-tag II and the N-terminus of INFa2b.

SEQ ID NO: 32 shows the nucleic acid sequence of pASK-IFNa2b.

SEQ ID NO: 33 shows a nucleic acid sequence stretch (upper/coding strand) encoding the C-terminus of Strep-tag II and the N-terminus of IFNa2b after insertion of one PA #1 polymer sequence cassette.

SEQ ID NO: 34 shows a nucleic acid sequence stretch (lower/non-coding strand) of the C-terminus of Strep-tag II and the N-terminus of IFNa2b after insertion of one PA #1 polymer sequence cassette.

SEQ ID NO: 35 shows an amino acid sequence stretch of the C-terminus of Strep-tag II and the N-terminus of IFNa2b ater fusion with one PA #1 polymer cassette.

SEQ ID NO: 36 shows the amino acid sequence of IFNa2b and Strep-tag II fused with the PA #1(200) polymer as encoded on pPA #1(200)-IFNa2b.

SEQ ID NO: 37 shows the nucleic acid sequence of pPA #1(200)-IFNa2b.

SEQ ID NO: 38 shows a nucleic acid sequence stretch (upper/coding strand) on pASK75-His6-hGH encoding the amino acid sequence around the N-terminus of His6-hGH.

SEQ ID NO: 39 shows a nucleic acid sequence stretch (lower/non-coding strand) on pASK75-His6-hGH encoding the amino acid sequence around the N-terminus of hGH.

SEQ ID NO: 40 shows an amino acid sequence stretch of the N-terminus of His6-hGH as encoded on pASK75-His6-hGH.

SEQ ID NO: 41 shows the nucleic acid sequence of pASK75-His6-hGH.

SEQ ID NO: 42 shows a nucleic acid sequence (upper/coding-strand) stretch encoding amino acid sequence of the N-terminus of His6-hGH after insertion of the PA #1(20) polymer.

SEQ ID NO: 43 shows a nucleic acid sequence (lower/non-coding strand) encoding the N-terminus of hGH after insertion of one PA #1 polymer sequence cassette.

SEQ ID NO: 44 shows the amino acid sequence of the N-terminus of His6-hGH after insertion of the PA #1(20) polymer.

SEQ ID NO: 45 shows the amino acid sequence of mature His6-PA #1(200)-hGH as encoded on pASK75-His6-PA #1(200)-hGH.

SEQ ID NO: 46 shows the nucleic acid sequence of pASK75-His6-PA #1(200)-hGH.

SEQ ID NO: 47 shows the amino acid sequence of His6-PA #1(200)-hGH as encoded on pCHO-PA #1(200)-hGH.

SEQ ID NO: 48 shows the nucleic acid sequence of pCHO-PA #1(200)-hGH.

SEQ ID NO: 49 shows the nucleic acid sequence of pCHO-hGH.

SEQ ID NO: 50 shows the nucleic acid sequence of pCHO.

SEQ ID NO: 51 shows the amino acid sequence of P1A1.

SEQ ID NO: 52 shows the nucleic acid sequence of upper/coding strand oligodesoxynucleotide used for the generation of the building block for P1A1.

SEQ ID NO: 53 shows the nucleic acid sequence of lower/non-coding strand oligodesoxynucleotide used for the generation of the building block for P1A1.

SEQ ID NO: 54 shows the nucleic acid sequence of upper/coding strand oligodesoxynucleotide used for the generation of the building block for P1A3.

SEQ ID NO: 55 shows the nucleic acid sequence of lower/non-coding strand oligodesoxynucleotide used for the generation of the building block for P1A3.

SEQ ID NO: 56 shows the amino acid sequence of the Fab light chain fused with the P1A1 (200) polymer as encoded on pFab-P1A1(200).

SEQ ID NO: 57 shows the amino acid sequence of the Fab light chain fused with the P1A3(200) polymer as encoded on pFab-P1A3(200).

SEQ ID NO: 58 shows the nucleic acid sequence of pFab-P1A1(200).

SEQ ID NO: 59 shows the acid sequence of pFab-P1A3(200).

SEQ ID NO: 60 shows the nucleic acid sequence of pSUMO-PA #1(200).

SEQ ID NO: 61 shows the PA #1(200) polypeptide/polymer used for the preparation of drug conjugates (made by ligation of 10 20mer encoding gene cassettes, including one additional C-terminal Ala residue resulting from the downstream ligation site. 

The invention claimed is:
 1. A nucleic acid molecule encoding a random coil polypeptide consisting of proline and alanine amino acid residues, wherein the random coil consists of at least 150 proline (Pro) and alanine (Ala) amino acid residues; wherein the random coil polypeptide can be incorporated into a drug conjugate comprising the random coil polypeptide conjugated to a drug selected from the group consisting of (a) a biologically active protein or a polypeptide with biological activity and (b) a small molecule drug.
 2. A vector comprising the nucleic acid molecule of claim
 1. 3. A host cell comprising the nucleic acid molecule of claim
 1. 4. The host cell according to claim 3, wherein said host cell is a eukaryotic host cell.
 5. The host cell according to claim 4, wherein said eukaryotic host cell is a fungal or animal cell.
 6. The nucleic acid molecule of claim 1, wherein said random coil polypeptide consists of 150 to 3000 amino acid residues.
 7. The nucleic acid molecule of claim 1, wherein said proline residues constitute more than 10% and less than 75% of the amino acid sequence.
 8. The nucleic acid molecule of claim 1, wherein no more than 6 consecutive amino acid residues are identical.
 9. The nucleic acid molecule of claim 1, wherein said random coil polypeptide comprises an amino acid sequence selected from the group consisting of (SEQ ID NO: 1) AAPAAPAPAAPAAPAPAAPA; (SEQ ID NO: 2) AAPAAAPAPAAPAAPAPAAP; (SEQ ID NO: 3) AAAPAAAPAAAPAAAPAAAP; (SEQ ID NO: 4) AAPAAPAAPAAPAAPAAPAAPAAP; (SEQ ID NO: 5) APAAAPAPAAAPAPAAAPAPAAAP; (SEQ ID NO: 6) AAAPAAPAAPPAAAAPAAPAAPPA; and (SEQ ID NO: 51) APAPAPAPAPAPAPAPAPAP

and circular permuted versions or (a) multimers(s) of these sequences.
 10. The nucleic acid molecule of claim 1, wherein said polypeptide with biological activity is selected from the group consisting of binding proteins, antibody fragments, cytokines, growth factors, hormones, and enzymes.
 11. The nucleic acid molecule of claim 1, wherein said polypeptide with biological activity is selected from the group consisting of antibodies, Fab fragments, F(ab′) 2 fragments, CDR-derived peptidomimetics, single chain variable fragments (scFv), domain antibodies, lectins, immunoglobulin domains, fibronectin domains, protein A domains, SH3 domains, ankyrin repeat domains, and lipocalins.
 12. The nucleic acid molecule of claim 1, wherein said biologically active protein is selected from the group consisting of granulocyte colony stimulating factor, human growth hormone, alpha-interferon, beta-interferon, gamma-interferon, tumor necrosis factor, erythropoietin, coagulation factor VIII, gp120/gp160, soluble tumor necrosis factor I and II receptor, reteplase, exendin-4, anakinra, interleukin-2, neutrophil gelatinase-associated lipocalin, follicle-stimulating hormone, glucocerebrosidase, thymosin alpha 1, glucagon, somatostatin, adenosine deaminase, interleukine 11, coagulation factor Vila, coagulation factor IX, hematide, lambda-interferon, leptin, interleukin-22 receptor subunit alpha (IL-22ra), interleukin-22, hyaluronidase, fibroblast growth factor 18, fibroblast growth factor 21, glucagon-like peptide 1, osteoprotegerin, IL-18 binding protein, growth hormone releasing factor, soluble TACI receptor, thrombospondin-1, soluble VEGF receptor Flt-1, and IL-4 mutein.
 13. The nucleic acid molecule of claim 1, whereby said random coil polypeptide mediates an increased in vivo and/or in vitro stability of said drug conjugate.
 14. The nucleic acid molecule of claim 13, wherein said increased in vivo stability is a prolonged plasma half-life of said drug conjugate when compared to the stability of a control polypeptide or a control conjugate lacking said random coil polypeptide.
 15. The nucleic acid molecule according to claim 1, wherein said small molecule drug is selected from the group consisting of digoxigenin, fluorescein, doxorubicin, calicheamicin, camptothecin, fumagillin, dexamethasone, geldanamycin, paclitaxel, docetaxel, irinotecan, cyclosporine, buprenorphine, naltrexone, naloxone, vindesine, vancomycin, risperidone, aripiprazole, palonosetron, granisetron, cytarabine NX1838, leuprolide, goserelin, buserelin, octreotide, teduglutide, cilengitide, abarelix, enfuvirtide, ghrelin, alpha 4 integrin inhibitors, antisense nucleic acids, small interference RNAs, micro RNAs, steroids, DNA or RNA aptamers, peptides, and peptidomimetics.
 16. The nucleic acid molecule according to claim 1, wherein the biologically active protein is selected from the group consisting of binding proteins, antibody fragments, cytokines, growth factors, hormones, and enzymes.
 17. A nucleic acid molecule encoding a drug conjugate, the drug conjugate comprising (i) a random coil polypeptide consisting of proline and alanine amino acid residues, wherein the random coil consists of at least 150 proline (Pro) and alanine (Ala) amino acid residues; and (ii) a biologically active protein or a polypeptide with biological activity.
 18. The nucleic acid molecule of claim 17, wherein the random coil polypeptide is encoded before or behind the biologically active protein or polypeptide with biological activity in a 5′ to 3′ orientation within the nucleic acid molecule.
 19. The nucleic acid molecule of claim 17 further comprising a protease and/or a chemical cleavage site and/or a recognition site between the random coil polypeptide and the biologically active protein or polypeptide with biological activity.
 20. The nucleic acid molecule according to claim 17 wherein the biologically active protein is selected from the group consisting of binding proteins, antibody fragments, cytokines, growth factors, hormones, and enzymes.
 21. The nucleic acid molecule according to claim 17 further comprising: (i) a nucleic acid sequence encoding a translated amino acid and/or a leader sequence; and (ii) a translational stop codon.
 22. A nucleic acid molecule encoding a random coil polypeptide consisting of proline and alanine amino acid residues, wherein the random coil polypeptide consists of at least 150 proline (Pro) and alanine (Ala) amino acid residues, said nucleic acid molecule comprising (i) a nucleic acid sequence encoding a translated amino acid and/or leader sequence; (ii) a nucleic acid sequence encoding the random coil polypeptide; and (iii) a translational stop codon.
 23. The nucleic acid molecule of claim 22 further comprising between (i) and (ii) a protease and/or a chemical cleavage site and/or a recognition site.
 24. A method for the preparation of a random coil polypeptide consisting of proline and alanine amino acid residues, wherein the random coil consists of at least 150 proline (Pro) and alanine (Ala) amino acid residues, and wherein the random coil polypeptide is conjugated to a drug selected from the group consisting of (a) a biologically active protein or a polypeptide with biological activity and (b) a small molecule drug, said method comprising culturing a host cell comprising a nucleic acid molecule encoding the random coil polypeptide or a vector comprising the nucleic acid, and isolating said random coil polypeptide from the culture or from said cell.
 25. The method of claim 24 further comprising conjugating the random coil polypeptide to the drug.
 26. The method of claim 25, wherein conjugating comprises a chemical linkage or coupling.
 27. A method for the production of a protein conjugate comprising: (i) a random coil polypeptide consisting of proline and alanine amino acid residues, wherein the random coil consists of at least 150 proline (Pro) and alanine (Ala) amino acid residues, and (ii) a biologically active protein or a polypeptide with biological activity, said method comprising cultivating a host cell comprising a nucleic acid molecule encoding the protein conjugate or a vector comprising the nucleic acid, and isolating the protein conjugate from the culture or from the host cell.
 28. The method of claim 27, wherein the protein conjugate is isolated from the growth medium or the culture medium, cellular lysates, cellular membrane fractions, or periplasm of the host cell. 